JP2004105173A - Prophylactic/remedy for respiratory disease - Google Patents

Abstract

<P>PROBLEM TO BE SOLVED: To develop an excellent prophylactic/remedy and diagnostic agent for respiratory diseases, scarcely having side effects. <P>SOLUTION: A compound which inhibits activity of a protein having an amino acid sequence identical or substantially identical to the amino acid sequence expressed by a specific sequence or a salt of the compound, another compound which inhibits expression of a gene of the protein, an antisense nucleotide which contains a base sequence complementary or substantially complementary to the base sequence of a DNA encoding the protein or its partial peptide or contains a part of the base sequence, an antibody to the protein or its partial peptide, etc., is used as the prophylactic/remedy for the respiratory diseases, etc. <P>COPYRIGHT: (C)2004,JPO

Description

【００７３】
本願明細書の配列表の配列番号は、以下の配列を示す。
〔配列番号：１〕
ヒトｎｍｂのアミノ酸配列を示す。
〔配列番号：２〕
配列番号：１で表されるアミノ酸配列を有するヒトｎｍｂをコードするＤＮＡの塩基配列を示す。
〔配列番号：３〕
マウスＤｅｎｄｒｉｔｉｃ　ｃｅｌｌ−ａｓｓｏｃｉａｔｅｄ　ｔｒａｎｓｍｅｍｂｒａｎｅ　ｐｒｏｔｅｉｎ　（ＤＣ−ＨＩＬ）のアミノ酸配列を示す。
〔配列番号：４〕
配列番号：３で表されるアミノ酸配列を有するマウスＤＣ−ＨＩＬをコードするＤＮＡの塩基配列を示す。
〔配列番号：５〕
実施例２および３で用いられたプライマーの塩基配列を示す。
〔配列番号：６〕
実施例２および３で用いられたプライマーの塩基配列を示す。
〔配列番号：７〕
実施例２および３で用いられたプライマーの塩基配列を示す。
〔配列番号：８〕
実施例２および３で用いられたプライマーの塩基配列を示す。
【００７４】
以下において、実施例により本発明をより具体的にするが、この発明はこれらに限定されるものではない。
【実施例】
実施例１
（１）タバコ煙曝露ＣＯＰＤモデルマウスの作製
ＣＯＰＤモデルは、Ｃ５７ＢＬ／６Ｎマウス（６週齡、日本チャールスリバー）にＫｅｎｔｕｃｋｙ　Ｒｅｆｅｒｅｎｃｅ　Ｃｉｇａｒｅｔｔｅ　１Ｒ１から発生する主流煙を、１〜４時間／日、５日／週ずつ計６ヶ月間吸入させて作製した。すなわち、Ｋｅｎｔｕｃｋｙ　Ｒｅｆｅｒｅｎｃｅ　Ｃｉｇａｒｅｔｔｅ　１Ｒ１をタバコ煙発生装置（ＳＧ−２００、柴田科学株式会社）に装着し、３５　ｍｌ／ｐｕｆｆ、１０　ｐｕｆｆ／ｍｉｎ、２５　ｐｕｆｆ／ｃｉｇａｒｅｔｔｅの条件で主流煙を採取した。得られた主流煙を空気で３％（Ｖ／Ｖ）に希釈した後に、マウスを入れたアクリル製の曝露チャンバーに送気し、自発呼吸下のマウスに所定の時間タバコ煙を吸入させた。なお、コントロール群には正常マウスを用いた。マウスの肺機能は摘出肺の圧−容量曲線を用いて評価した。すなわち、１ヶ月、３ヶ月および６ヶ月間のタバコ煙曝露が終了した翌日に、マウスをペントバルビタール（７０　ｍｇ／ｋｇ，　ｉ．ｐ．）で麻酔した後、頸部を切開し、気管にカニューレ（サーフロー留置針、１８Ｇ）を挿入した。この気管カニューレに人工呼吸器（Ｈａｒｖａｒｄ社）を連結し、横隔膜切除下で、９９．９９５％　Ｏ_２により１０分間人工呼吸を施した。なお、その際の気道内圧変化が１０　ｃｍ　Ｈ_２Ｏとなるように換気量を調節した。人工呼吸終了後、気管を動脈クリップで閉じて肺内のｄｅｇａｓｓｉｎｇを行った後、肺を摘出した。この摘出肺に、０〜２５　ｃｍ　Ｈ_２Ｏの圧力でホルマリン緩衝液を順次注入して、５　ｃｍ　Ｈ_２Ｏごとの肺の体積をｐｒｅｔｈｙｓｍｏｇｒａｐｈ　（Ｕｇｏｂａｓｉｌ社）を用いて測定し、摘出肺の圧−容量曲線を求めた。結果を図１に示す。
【００７５】
（２）タバコ煙曝露ＣＯＰＤモデルマウス肺で発現変動する遺伝子の探索
タバコ煙曝露ＣＯＰＤモデルマウス肺で特異的に発現変動している遺伝子を明らかにするため、最終曝露が終了した翌日にマウスをペントバルビタール麻酔により致死させ、気管支肺胞洗浄を施行した後に肺を摘出した。摘出肺は液体窒素中で凍結させ、凍結組織破砕装置で粉砕した後に、その湿重量の１０倍量に相当するＩｓｏｇｅｎ（和光純薬社製）に浸した。１ヶ月タバコ煙曝露群（ｎ＝１０）、そのコントロール群（ｎ＝６）、３ヶ月タバコ煙曝露群（ｎ＝８）、そのコントロール群（ｎ＝８）、６ヶ月タバコ煙曝露群（ｎ＝８）、そのコントロール群（ｎ＝８）からＩＳＯＧＥＮを用いて、添付のマニュアルに従って抽出したｔｏｔａｌ　ＲＮＡを材料とし、ｏｌｉｇｏｎｕｃｌｅｏｔｉｄｅ　ｍｉｃｒｏａｒｒａｙ　（Ｍｏｕｓｅ　Ｇｅｎｏｍｅ　Ｕ９４Ａ，　Ｕ９４Ｂ，　Ｕ９４Ｃ；　Ａｆｆｙｍｅｔｒｉｘ社）　を用いて遺伝子発現解析を行った。
実験方法は、Ａｆｆｙｍｅｔｒｉｘ社の実験手引き書　（Ｅｘｐｒｅｓｓｉｏｎ　ａｎａｌｙｓｉｓ　ｔｅｃｈｎｉｃａｌ　ｍａｎｕａｌ）　に従った。その結果、タバコ煙曝露ＣＯＰＤモデルマウスで特異的に発現が増加する遺伝子としてａｆｆｙｍｅｔｒｉｘ　Ｎｏ．　１０８８２２＿ａｔが検出された。この配列を基にＢＬＡＳＴ検索をしたところ、この遺伝子はマウスＤｅｎｄｒｉｔｉｃ　ｃｅｌｌ−ａｓｓｏｃｉａｔｅｄ　ｔｒａｎｓｍｅｍｂｒａｎｅ　ｐｒｏｔｅｉｎ　（ＤＣ−ＨＩＬ）（マウスｎｍｂと称することもある）をコードしていた。また、そのヒトカウンターパートは、ヒトｎｍｂ（配列番号：１）であると判明した。
【００７６】
実施例２
定量的ＲＴ−ＰＣＲ法による発現変動の確認
ＤＣ−ＨＩＬ遺伝子の発現変動が個体レベルでも顕著に認められることを確認するため、定量的ＲＴ−ＰＣＲ法により、個体毎の発現を調べた。
マウス肺組織から調製したｔｏｔａｌ　ＲＮＡ　２００ｎｇを出発材料としてＴａｑＭａｎ　Ｇｏｌｄ　ＲＴ−ＰＣＲ　Ｋｉｔ（アプライドバイオシステムズ社製）を用いて５０μｌの反応液中で逆転写反応によりｃＤＮＡを合成した。反応液を蒸留水で５倍に希釈した後、そのうちの７μｌを用いてＡＢＩ　ＰＲＩＳＭ　７９００シークエンスディテクター（アプライドバイオシステムズ社製）とＱｕａｎｔｉＴｅｃｔ　ＳＹＢＲ　Ｇｒｅｅｎ　ＰＣＲ　Ｋｉｔ（ＱＩＡＧＥＮ社製）を用いたリアルタイム定量的ＰＣＲ法により、マウスＤＣ−ＨＩＬ遺伝子コピー数を測定した。遺伝子量検出に用いたプライマー〔プライマー１（配列番号：５）およびプライマー２（配列番号：６）〕はマウスＤＣ−ＨＩＬ遺伝子の塩基配列〔ＧｅｎＢａｎｋ　Ａｃｃｅｓｓｉｏｎ　Ｎｕｍｂｅｒ：　ＡＦ３２２０５４〕からＰｒｉｍｅｒ　Ｅｘｐｒｅｓｓプログラムを用いて設計した。コピー数算出のための標準サンプルとしては、マウス肺組織から抽出したｔｏｔａｌ　ＲＮＡを鋳型にプライマー３（配列番号：７）およびプライマー４（配列番号：８）を用いて、ＲＴ−ＰＣＲ法により増幅した５１５塩基対からなるＤＮＡ断片の濃度をＳｐｅｃｔｒｏｐｈｏｔｏｍｅｔｅｒ（ベックマン社製）により、測定し、段階希釈することにより調製した。同様にハウスキーピング遺伝子としてＧＡＰＤＨ遺伝子のコピー数を測定した。また、非特異的な増幅を除去するために逆転写酵素を含まないサンプルも同様に処理し、次式より、ｔｏｔａｌ　ＲＮＡあたりの遺伝子コピー数を求め、タバコ煙曝露ＣＯＰＤモデルマウス肺とコントロールマウス肺の個体毎の発現を比較した。
（逆転写酵素含有サンプル中のＤＣ−ＨＩＬ遺伝子コピー数／ＧＡＰＤＨ遺伝子コピー数）−（逆転写酵素非含有サンプル中のＤＣ−ＨＩＬ遺伝子コピー数／ＧＡＰＤＨ遺伝子コピー数）＝（ＤＣ−ＨＩＬ遺伝子発現量）
結果を図２に示す。
これより、マウスＤＣ−ＨＩＬ遺伝子（配列番号：４）の発現がＣＯＰＤモデルマウス肺で有意に増加している（＊＊ｐ≦０．０１）ことがわかった。
【００７７】
実施例３
マウスＤＣ−ＨＩＬ遺伝子産物の組織分布の解析
マウスの各組織（骨髄、平滑筋、前立腺、胸腺、胃、子宮、心臓、脳、脾臓、肺、肝臓、腎臓、精巣）のｃＤＮＡ（Ｍｏｕｓｅ　ＭＴＣ　ｐａｎｅｌ　ＩおよびＭｏｕｓｅ　ＭＴＣ　ｐａｎｅｌＩＩ：クロンテック社製）およびタバコ煙曝露モデルマウス肺およびコントロールマウス肺ｃＤＮＡ（１，　３，　６ヶ月処理混合群）を鋳型として、ＡＢＩ　ＰＲＩＳＭ　７９００シークエンスディテクター（アプライドバイオシステムズ社製）とＱｕａｎｔｉＴｅｃｔ　ＳＹＢＲ　Ｇｒｅｅｎ　ＰＣＲ　Ｋｉｔ（ＱＩＡＧＥＮ社製）を用いたリアルタイム定量的ＰＣＲ法により、マウスＤＣ−ＨＩＬ遺伝子発現分布を調べた。遺伝子量検出に用いたプライマー〔プライマー１（配列番号：５）およびプライマー２（配列番号：６）〕はマウスＤＣ−ＨＩＬ遺伝子の塩基配列〔ＧｅｎＢａｎｋ　Ａｃｃｅｓｓｉｏｎ　Ｎｕｍｂｅｒ：　ＡＦ３２２０５４〕からＰｒｉｍｅｒ　Ｅｘｐｒｅｓｓプログラムを用いて設計した。コピー数算出のための標準サンプルとしては、マウス肺組織から抽出したｔｏｔａｌ　ＲＮＡを鋳型にプライマー３（配列番号：７）およびプライマー４（配列番号：８）を用いて、ＲＴ−ＰＣＲ法により増幅した５１５塩基対からなるＤＮＡ断片の濃度をＳｐｅｃｔｒｏｐｈｏｔｏｍｅｔｅｒ（ベックマン社製）により、測定し、段階希釈することにより調製した。同様にハウスキーピング遺伝子としてＧＡＰＤＨ遺伝子のコピー数を測定した。また、非特異的な増幅を除去するために逆転写酵素を含まないサンプルも同様に処理し、次式より、ｔｏｔａｌ　ＲＮＡあたりの遺伝子コピー数を求めることにより発現量を求めた。
（逆転写酵素含有サンプル中のＤＣ−ＨＩＬ遺伝子コピー数／ＧＡＰＤＨ遺伝子コピー数）−（逆転写酵素非含有サンプル中のＤＣ−ＨＩＬ遺伝子コピー数／ＧＡＰＤＨ遺伝子コピー数）＝（ＤＣ−ＨＩＬ遺伝子発現量）
結果を図３に示す。
その結果、マウスＤＣ−ＨＩＬ遺伝子産物（ｍＲＮＡ）は肺に特異的に発現していることが判明した。
【００７８】
実施例４
（１）エラスターゼ誘発ＣＯＰＤモデルマウスの作製
ＣＯＰＤモデルは、Ｃ５７ＢＬ／６Ｎマウス（８週齡、日本チャールスリバー）にブタ膵臓エラスターゼ溶液（和光純薬）（６　ｕｎｉｔｓ／５０μＬ／マウス）をハロタン麻酔下にて点鼻投与して作製した。なお、コントロール群には生理食塩液点鼻マウスを用いた。マウスの肺機能は摘出肺の圧−容量曲線を用いて評価した。すなわち、エラスターゼ投与１日、３日、７日、１４日、２１日および３５日後にマウスをペントバルビタール（７０　ｍｇ／ｋｇ　腹腔内投与）で麻酔した後、頸部を切開し気管にカニューレ（サーフロー留置針、１８Ｇ）を挿入した。この気管カニューレに人工呼吸器（Ｈａｒｖａｒｄ社製）を連結し、横隔膜切除下で　９９．９９５％　Ｏ_２を用いて１０分間人工呼吸を施した。なお、その際の気道内負荷圧が１０　ｃｍ　Ｈ_２Ｏとなるように換気量を調節した。人工呼吸終了後、気管を動脈クリップで閉じて肺内のｄｅｇａｓｓｉｎｇを行った後、肺を摘出した。この摘出肺に、０〜２５　ｃｍ　Ｈ_２Ｏの負荷圧下でホルマリン緩衝液を順次注入して、５　ｃｍ　Ｈ_２Ｏごとの肺の体積をｐｌｅｔｈｙｓｍｏｇｒａｐｈ　（Ｕｇｏｂａｓｉｌ社製）を用いて測定し、摘出肺の圧−容量曲線を求めた。また、以下の式に従い、肺の広がり易さの指標としてコンプライアンス値を算出した。
｛２５　ｃｍ　Ｈ_２Ｏの負荷圧下での肺容量増加量（ｍＬ）｝／２５　（ｃｍＨ_２Ｏ）　＝　コンプライアンス値
結果を図４および図５に示す。
（２）エラスターゼ誘発ＣＯＰＤモデルマウス肺で発現変動する遺伝子の探索
エラスターゼ誘発ＣＯＰＤモデルマウス肺で特異的に発現変動している遺伝子を明らかにするため、エラスターゼ投与１日、３日、７日、１４日、２１日および３５日後にマウスをペントバルビタール麻酔により致死させ肺を摘出した。摘出肺は液体窒素中で凍結させ、凍結組織破砕装置で粉砕した後に、その湿重量の１０倍量に相当するＩＳＯＧＥＮ（和光純薬）に浸した。エラスターゼ投与１日後群、エラスターゼ投与３日後群、エラスターゼ投与７日後群、エラスターゼ投与１４日後群、エラスターゼ投与２１日後群、エラスターゼ投与３５日後群（いずれもｎ＝６）およびそれらコントロール群（いずれもｎ＝６）からＩＳＯＧＥＮを用いて、添付のマニュアルに従ってｔｏｔａｌ　ＲＮＡを調製した。
マウス肺組織から調製したｔｏｔａｌ　ＲＮＡ　１μｇを出発材料としてＭ−ＭＬＶ　Ｒｅｖｅｒｓｅ　Ｔｒａｎｓｃｒｉｐｔａｓｅ　（インビトロジェン社製）を用いて５０μｌの反応液中で逆転写反応によりｃＤＮＡを合成した。その反応液を用いてＡＢＩ　ＰＲＩＳＭ　７７００シークエンスディテクター（アプライドバイオシステムズ社製）を用いたリアルタイム定量的ＰＣＲ法により、マウスＤＣ−ＨＩＬ遺伝子量を測定した。遺伝子量検出に用いたプライマー〔プライマー１（配列番号：５）およびプライマー２（配列番号：６）〕はマウスＤＣ−ＨＩＬ遺伝子の塩基配列（ＧｅｎＢａｎｋ　Ａｃｃｅｓｓｉｏｎ　Ｎｕｍｂｅｒ：　ＡＦ３２２０５４）からＰｒｉｍｅｒ　Ｅｘｐｒｅｓｓプログラムを用いて設計した。同様にハウスキーピング遺伝子として１８ＳリボゾーマルＲＮＡ遺伝子の遺伝子量を測定した。次式より、１８ＳリボゾーマルＲＮＡ遺伝子発現量あたりのＤＣ−ＨＩＬ遺伝子発現量を求め、エラスターゼ誘発ＣＯＰＤモデルマウス肺とコントロールマウス肺の個体毎の発現を比較した。
（ＤＣ−ＨＩＬ遺伝子発現量／１８ＳリボゾーマルＲＮＡ遺伝子発現量）＝（ＤＣ−ＨＩＬ遺伝子発現量）
結果を図６に示す。
これより、ＤＣ−ＨＩＬ遺伝子（配列番号：４）の発現がエラスターゼ誘発ＣＯＰＤモデルマウス肺で有意に増加している（＊＊ｐ≦０．０１）ことがわかった。
【００７９】
【発明の効果】
本発明のタンパク質およびポリヌクレオチドは、例えば呼吸器疾患〔例、慢性閉塞性肺疾患（慢性気管支炎、肺気腫）、びまん性汎細気管支炎、気管支喘息、嚢胞性線維症、過敏性肺炎、肺線維症など〕、鼻炎（例、アレルギー性鼻炎、花粉症、急性鼻炎、慢性鼻炎、肥厚性鼻炎、萎縮性鼻炎、乾燥性前鼻炎、血管運動性鼻炎、壊疽性鼻炎、副鼻腔炎など）、免疫疾患（例、重症筋無力症、糸球体腎炎、多発性硬化症、シェーグレン症候群、インスリン抵抗性糖尿病、慢性関節リウマチ、全身性エリテマトーデス、アトピー性皮膚炎、白血球異常、脾機能不全または胸腺異常にともなう免疫不全など）、炎症性腸疾患、アレルギー性結膜炎などの診断マーカー等として有用であり、該タンパク質、ポリヌクレオチドまたは該タンパク質に対する抗体などを用いるスクリーニングにより得られる調節剤（好ましくは阻害剤）、該タンパク質に対する中和抗体などは、例えば、呼吸器疾患〔例、慢性閉塞性肺疾患（慢性気管支炎、肺気腫）、びまん性汎細気管支炎、気管支喘息、嚢胞性線維症、過敏性肺炎、肺線維症など〕、鼻炎（例、アレルギー性鼻炎、花粉症、急性鼻炎、慢性鼻炎、肥厚性鼻炎、萎縮性鼻炎、乾燥性前鼻炎、血管運動性鼻炎、壊疽性鼻炎、副鼻腔炎など）、免疫疾患（例、重症筋無力症、糸球体腎炎、多発性硬化症、シェーグレン症候群、インスリン抵抗性糖尿病、慢性関節リウマチ、全身性エリテマトーデス、アトピー性皮膚炎、白血球異常、脾機能不全または胸腺異常にともなう免疫不全など）、炎症性腸疾患、アレルギー性結膜炎などの予防・治療剤として使用することができる。好ましくは、呼吸器疾患などの予防・治療剤、さらに好ましくは慢性閉塞性肺疾患などの予防・治療剤、さらに好ましくは肺気腫などの予防・治療剤である。
また、本発明のアンチセンスポリヌクレオチドは、本発明のタンパク質の発現を抑制することができ、例えば、呼吸器疾患〔例、慢性閉塞性肺疾患（慢性気管支炎、肺気腫）、びまん性汎細気管支炎、気管支喘息、嚢胞性線維症、過敏性肺炎、肺線維症など〕、鼻炎（例、アレルギー性鼻炎、花粉症、急性鼻炎、慢性鼻炎、肥厚性鼻炎、萎縮性鼻炎、乾燥性前鼻炎、血管運動性鼻炎、壊疽性鼻炎、副鼻腔炎など）、免疫疾患（例、重症筋無力症、糸球体腎炎、多発性硬化症、シェーグレン症候群、インスリン抵抗性糖尿病、慢性関節リウマチ、全身性エリテマトーデス、アトピー性皮膚炎、白血球異常、脾機能不全または胸腺異常にともなう免疫不全など）、炎症性腸疾患、アレルギー性結膜炎などの予防・治療剤や診断薬として使用することができる。好ましくは、呼吸器疾患などの予防・治療剤、さらに好ましくは慢性閉塞性肺疾患などの予防・治療剤、さらに好ましくは肺気腫などの予防・治療剤である。
【００８０】
【配列表】

【図面の簡単な説明】
【図１】実施例１で得られたマウス摘出肺の圧−容量曲線を表す図である。図中、（ａ）の−●−は１ヶ月間のタバコ煙曝露マウス群（ｎ＝８）、−○−はコントロール群（ｎ＝７）を、（ｂ）の−●−は３ヶ月間のタバコ煙曝露マウス群（ｎ＝１０）、−○−はコントロール群（ｎ＝９）を、（ｃ）の−●−は６ヶ月間のタバコ煙曝露マウス群（ｎ＝１０）、−○−はコントロール群（ｎ＝９）を示す。＊＊はｐ≦０．０１を、＊はｐ≦０．０５を示す。
【図２】実施例２で得られたマウスＤＣ−ＨＩＬ遺伝子発現量の結果を表す図である。図中、横軸のＡは１ヶ月間のタバコ煙曝露マウス肺、Ｂはそのコントロールマウス肺、Ｃは３ヶ月間のタバコ煙曝露マウス肺、Ｄはそのコントロールマウス肺、Ｅは６ヶ月間のタバコ煙曝露マウス肺、Ｆはそのコントロールマウス肺を示す。
【図３】実施例３で得られたマウスＤＣ−ＨＩＬ遺伝子発現分布の結果を表す図である。
【図４】実施例４で得られたマウス摘出肺の圧−容量曲線を表す図である。図中、（ａ）の−■−はエラスターゼ投与１日後のマウス群（ｎ＝６）、−□−はコントロール群（ｎ＝６）を、（ｂ）の−■−はエラスターゼ投与７日後のモデルマウス群（ｎ＝５）、−□−はコントロール群（ｎ＝６）を、（ｃ）の−■−はエラスターゼ投与２１日後のモデルマウス群（ｎ＝６）、−□−はコントロール群（ｎ＝６）を示す。＊はｐ≦０．０５、＊＊はｐ≦０．０１を示す。
【図５】実施例４で得られたエラスターゼ投与後のマウス摘出肺のコンプライアンス値の経時的変化を表す図である。図中、横軸はエラスターゼ投与後の日数、縦軸はコンプライアンス値を示す。−■−はエラスターゼ投与マウス群（ｎ＝６）、−□−はコントロール群（ｎ＝６）を示す。＊はｐ≦０．０５、＊＊はｐ≦０．０１を示す。
【図６】実施例４で得られたエラスターゼ投与後のマウス肺組織でのＤＣ−ＨＩＬ遺伝子発現量の経時的変化を表す図である。図中、横軸はエラスターゼ投与後の日数、縦軸はＤＣ−ＨＩＬ遺伝子発現量を示す。−■−はエラスターゼ投与マウス群（ｎ＝６）、−□−はコントロール群（ｎ＝６）を示す。＊はｐ≦０．０５、＊＊はｐ≦０．０１を示す。[0001]
TECHNICAL FIELD OF THE INVENTION
The present invention relates to a prophylactic / therapeutic agent for respiratory diseases, a diagnostic agent, and the like.
[0002]
[Prior art]
Chronic obstructive pulmonary disease, chronic bronchitis, emphysema, diffuse panbronchiolitis, endogenous asthma, etc. It is thought to be.
It has been shown that smoking can be a definite etiology of chronic obstructive pulmonary disease. Smoking causes obstructive disorders, which depend on the number of cigarettes. The younger the age at which smoking starts, the easier it is to progress. In addition, a dose correlation between smoking and bronchial gland hyperplasia has been confirmed.
There are many reports in animal experiments that inhalation of tobacco can cause emphysema.
Pathological changes of chronic obstructive pulmonary disease (hereinafter, sometimes abbreviated as COPD) include specific abnormalities in three areas: central airway, peripheral airway, and lung parenchyma. Central airway lesions show changes in secretory tissue morphology such as hyperplasia of goblet cells, proliferation of cells in the submucosal glands, and hypertrophy. Regarding inflammatory cells, an increase in macrophages and activated T lymphocytes has been shown in the airway mucosa. Lesions in the bronchiole region include mucus embolism in the airway lumen, goblet cell dysplasia in the airway epithelium, inflammatory cell infiltration in the airway wall, smooth muscle hypertrophy, and fibrosis. Either change results in airway narrowing. In the alveolar parenchyma, emphysema lesions defined by destruction and disappearance of the alveoli and enlargement of the air space are observed. These are thought to involve a protease / antiprotease balance imbalance.
On the other hand, in order to comprehensively analyze gene expression, a microarray method in which cDNAs or oligonucleotides are immobilized has been developed, and techniques for finding disease-specific changes in gene expression have become widespread, and their usefulness has been confirmed. . For example, Affymetrix's GeneChip system is being widely used for diagnosing diseases such as cancer and finding drug discovery target genes. However, there is no report using this technique to find genes involved in the onset or progression of emphysema.
Recently, Dendritic cell-associated transmembrane protein (DC-HIL) has been cloned as a gene specifically expressed in Dendritic cells, and the protein is involved in adhesion to endothelial cells through binding to heparan sulfate proteoglycans and RGD sequences. (J. Biol. Chem., 276, 8125, 2001).
[Non-patent document 1]
Journal of Biological Chemistry 276, 8125, 2001
[0003]
[Problems to be solved by the invention]
There is a demand for the development of a prophylactic / therapeutic agent and a diagnostic agent for an excellent respiratory disease with few side effects (eg, chronic obstructive pulmonary disease).
[0004]
[Means for Solving the Problems]
The present inventors have conducted intensive studies in order to solve the above problems, and found a gene whose expression is significantly increased in lung tissue having emphysema lesions. Thus, the present invention has been completed.
[0005]
That is, the present invention
(1) A respiratory tract containing a compound or a salt thereof which inhibits the activity of a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof or a salt thereof Preventive and therapeutic agents for diseases,
(2) a protein or a partial peptide thereof having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, or a compound thereof or a salt thereof which inhibits the expression of a gene thereof; Prophylactic and therapeutic agents for respiratory diseases,
(3) a base complementary or substantially complementary to a base sequence of a polynucleotide encoding a protein or a partial peptide thereof containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 An antisense polynucleotide containing the sequence or a portion thereof,
(4) a medicine comprising the antisense polynucleotide according to (3),
(5) The medicament according to the above (4), which is a prophylactic / therapeutic agent for a respiratory disease.
(6) an antibody against a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof;
(7) a medicine comprising the antibody according to the above (6),
(8) The medicament according to the above (7), which is a prophylactic / therapeutic agent for a respiratory disease.
(9) a diagnostic agent comprising the antibody of (6) above,
(10) The diagnostic agent according to the above (9), which is a diagnostic agent for a respiratory disease.
(11) a diagnostic agent for a respiratory disease comprising a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof,
(12) a prophylactic / therapeutic agent for a respiratory disease, comprising a compound having a function of inhibiting heparan sulfate proteoglycan binding activity or a salt thereof;
(13) A prophylactic / therapeutic agent for a respiratory disease, characterized by using a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof. Screening method,
(13a) a method for screening a pharmaceutical compound, which comprises using a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof;
(13b) The pharmaceutical compound described above (13a), wherein the pharmaceutical compound is a compound for preventing or treating a respiratory disease, a compound used for preventing or treating a respiratory disease, and / or a compound having a preventive or treating effect for a respiratory disease. Described screening method,
(14) The screening method according to (13) above, wherein the tobacco smoke-exposed chronic obstructive pulmonary disease model mouse or the elastase-induced chronic obstructive pulmonary disease model mouse is used.
(15) A prophylactic / therapeutic agent for a respiratory disease comprising a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, or a partial peptide thereof or a salt thereof. Screening kit,
(15a) a kit for screening a pharmaceutical compound, which comprises a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof;
(15b) The above-mentioned (15a), wherein the pharmaceutical compound is a compound for preventing / treating a respiratory disease, a compound used for preventing / treating a respiratory disease, and / or a compound having a preventive / treating effect for a respiratory disease. The screening kit described,
(16) a prophylactic / therapeutic agent for a respiratory disease obtainable by using the screening method according to (13) or the screening kit according to (15);
(16a) a pharmaceutical compound obtainable using the screening method according to (13a) or the screening kit according to (15a);
(16b) The above-mentioned (16a), wherein the pharmaceutical compound is a compound for preventing / treating a respiratory disease, a compound used for preventing / treating a respiratory disease, and / or a compound having a preventive / treating effect for a respiratory disease. The compound or a salt thereof,
(16c) a prophylactic / therapeutic agent for a respiratory disease comprising the compound according to (16b) or a salt thereof,
(17) The prophylactic / therapeutic agent according to the above (16), wherein the respiratory disease is emphysema.
(18) Prevention / treatment of respiratory disease, characterized by using a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof. Agent screening method,
(18a) a method for screening a pharmaceutical compound, which comprises using a polynucleotide encoding a protein or a partial peptide thereof having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1,
(18b) The above-mentioned (18a), wherein the pharmaceutical compound is a compound for preventing or treating a respiratory disease, a compound used for preventing or treating a respiratory disease, and / or a compound having a preventive or treating effect for a respiratory disease. Described screening method,
(19) The screening method according to (18), wherein the tobacco smoke-exposed chronic obstructive pulmonary disease model mouse or elastase-induced chronic obstructive pulmonary disease model mouse is used.
(20) prevention of respiratory diseases characterized by containing a polynucleotide encoding a protein or a partial peptide thereof having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1; Kit for screening therapeutic agents,
(20a) for screening a pharmaceutical compound comprising a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof kit,
(20b) The above-mentioned (20a), wherein the pharmaceutical compound is a compound for preventing or treating respiratory disease, a compound used for preventing or treating respiratory disease, and / or a compound having a preventive or treating effect for respiratory disease. The screening kit described,
(21) a prophylactic / therapeutic agent for a respiratory disease obtainable by using the screening method according to (18) or the screening kit according to (20);
(21a) a pharmaceutical compound obtainable by using the screening method according to (18a) or the screening kit according to (20a);
(21b) The above-mentioned (21a), wherein the pharmaceutical compound is a compound for preventing / treating a respiratory disease, a compound used for preventing / treating a respiratory disease, and / or a compound having a preventive / treating effect for a respiratory disease. The compound or a salt thereof,
(21c) a prophylactic / therapeutic agent for a respiratory disease comprising the compound according to (21b) or a salt thereof,
(22) The prophylactic / therapeutic agent according to the above (21), wherein the respiratory disease is emphysema.
(23) a compound that inhibits the activity of a protein or a partial peptide thereof or a salt thereof, or a salt thereof, which contains the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, for a mammal; or A method for preventing or treating a respiratory disease, which comprises administering an effective amount of a compound that inhibits the expression of the protein gene or a salt thereof,
(24) Inhibits the activity of a protein containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof, or inhibits the gene expression of the protein A method for preventing and treating respiratory diseases,
(25) Activity of a protein containing an amino acid sequence identical or substantially identical to the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof or a salt thereof for producing a prophylactic / therapeutic agent for a respiratory disease And a salt thereof, or a compound inhibiting the expression of the protein gene or a salt thereof.
[0006]
BEST MODE FOR CARRYING OUT THE INVENTION
The protein containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 (hereinafter, sometimes referred to as the protein of the present invention or the protein used in the present invention) used in the present invention is Cells of humans and warm-blooded animals (eg, guinea pig, rat, mouse, chicken, rabbit, pig, sheep, cow, monkey, etc.) (eg, hepatocytes, spleen cells, nerve cells, glial cells, pancreatic β cells, bone marrow) Cells, mesangial cells, Langerhans cells, epidermal cells, epithelial cells, goblet cells, endothelial cells, smooth muscle cells, fibroblasts, fiber cells, muscle cells, adipocytes, immune cells (eg, macrophages, T cells, B cells, Natural killer cells, mast cells, neutrophils, basophils, eosinophils, monocytes), megakaryocytes, synovial cells, chondrocytes, osteocytes, osteoblasts, osteoclasts Mammary gland cells, hepatocytes or stromal cells, or precursors of these cells, stem cells or cancer cells) or any tissue in which these cells are present, for example, the brain, various parts of the brain (eg, olfactory bulb, amygdala, cerebrum) Basal sphere, hippocampus, thalamus, hypothalamus, cerebral cortex, medulla, cerebellum), spinal cord, pituitary, stomach, pancreas, kidney, liver, gonad, thyroid, gallbladder, bone marrow, adrenal gland, skin, muscle, lung, digestive tract ( Eg, large intestine, small intestine), blood vessels, heart, thymus, spleen, submandibular gland, peripheral blood, prostate, testis, ovary, placenta, uterus, bone, joint, skeletal muscle, etc. It may be a protein.
[0007]
As the amino acid sequence substantially identical to the amino acid sequence represented by SEQ ID NO: 1, about 50% or more, preferably about 60% or more, and more preferably about 70% Above, more preferably about 80% or more, particularly preferably about 90% or more, most preferably about 95% or more amino acid sequence having homology.
The homology of amino acid sequences was determined using the homology calculation algorithm NCBI BLAST (National Center for Biotechnology Information Basic Local Alignment Search Tool) under the following conditions (expected value = 10; gap allowed; matrix = BLOSUM62; filtering = BLOSUM62). Can be calculated.
Examples of the protein containing an amino acid sequence substantially the same as the amino acid sequence represented by SEQ ID NO: 1 include, for example, a protein containing the same amino acid sequence as the above-mentioned amino acid sequence represented by SEQ ID NO: 1. And proteins having substantially the same activity as the protein containing the amino acid sequence represented by SEQ ID NO: 1. Examples of the protein containing the amino acid sequence substantially identical to the amino acid sequence represented by SEQ ID NO: 1 include a protein containing the amino acid sequence represented by SEQ ID NO: 3, and the like.
[0008]
Examples of substantially equivalent activities include, for example, cell adhesion activity, heparan sulfate proteoglycan binding activity, and the like. Substantially homogenous indicates that the properties are homogenous (eg, physiologically or pharmacologically). Therefore, it is preferable that the cell adhesion activity, the heparan sulfate proteoglycan binding activity, and the like are equivalent (eg, about 0.01 to 100 times, preferably about 0.1 to 10 times, more preferably 0.5 to 2 times). However, the quantitative factors such as the degree of these activities and the molecular weight of the protein may be different.
Cell adhesion activity and heparan sulfate proteoglycan binding activity can be measured by a method known per se, for example, J. Am. Biol. Chem. 276 (11), 8125-8134, 2001 or a method analogous thereto.
Specifically, the cell adhesion activity is measured by mixing a fusion protein of the extracellular region of the protein of the present invention with an immunoglobulin Fc region and an endothelial cell, and then using a labeled (eg, enzyme-labeled) Fc region-recognizing antibody. After the reaction, the substrate is added, the enzyme reaction is performed, and the activity is measured. This reaction is performed in an appropriate buffer. Perform the washing operation as necessary. The measurement of the enzyme reaction is performed according to a known method using a microplate reader or the like.
The extracellular region of the protein of the present invention includes, for example, a peptide having the 1st to 319th amino acid sequence of the amino acid sequence represented by SEQ ID NO: 1. Fusion proteins between the extracellular region of the protein of the present invention and the immunoglobulin Fc region can be prepared by known methods, for example, as described in J. Am. Biol. Chem. 276 (11), 8125-8134, 2001 or a method analogous thereto. As the endothelial cells, for example, vascular endothelial cells and the like are used.
Heparan sulfate proteoglycan binding activity was determined by reacting a heparin-BSA-immobilized microplate and a fusion protein of the extracellular region of the protein of the present invention with the Fc region of an immunoglobulin (for example, enzyme labeling). A) reacting with an antibody recognizing the Fc region, adding a substrate, causing an enzymatic reaction, and measuring the activity. This reaction is performed in an appropriate buffer. Perform the washing operation as necessary. The measurement of the enzyme reaction is performed according to a known method using a microplate reader or the like.
The extracellular region of the protein of the present invention includes, for example, a peptide having the 1st to 319th amino acid sequence of the amino acid sequence represented by SEQ ID NO: 1. Fusion proteins between the extracellular region of the protein of the present invention and the immunoglobulin Fc region can be prepared by known methods, for example, as described in J. Am. Biol. Chem. 276 (11), 8125-8134, 2001 or a method analogous thereto.
[0009]
Examples of the protein used in the present invention include (1) (1) one or two or more (for example, about 1 to 100, preferably 1 to 30) amino acids in the amino acid sequence represented by SEQ ID NO: 1. (Preferably about 1 to 10, more preferably number (1 to 5) amino acids). (2) 1 or 2 or more amino acids in the amino acid sequence represented by SEQ ID NO: 1 ( For example, an amino acid sequence to which about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, and more preferably a number (1 to 5) amino acids have been added; One or more amino acids (for example, about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, and more preferably a number (1 to 5)) are inserted into the represented amino acid sequence. Amino acid sequence {Circle around (4)} One or two or more amino acids in the amino acid sequence represented by SEQ ID NO: 1 (for example, about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, more preferably So-called muteins, such as a protein containing an amino acid sequence in which 〜5) amino acids are substituted with another amino acid, or (5) a protein containing an amino acid sequence obtained by combining them.
(2) {circle around (1)} One or two or more amino acids in the amino acid sequence represented by SEQ ID NO: 3 (for example, about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, more preferably about 1 to 10) An amino acid sequence in which several (1 to 5) amino acids have been deleted; (2) one or more amino acids (for example, about 1 to 100, preferably 1 to 30) in the amino acid sequence represented by SEQ ID NO: 3 (Preferably about 1 to 10, more preferably number (1 to 5) amino acids), and (3) one or more amino acids (for example, An amino acid sequence into which about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, and more preferably a number (1 to 5) amino acids have been inserted; (4) SEQ ID NO: 3 One or more of the amino acid sequences represented An amino acid sequence in which two or more (eg, about 1 to 100, preferably about 1 to 30, preferably about 1 to 10, and more preferably number (1 to 5) amino acids) have been substituted with other amino acids Or (5) so-called muteins such as proteins containing an amino acid sequence obtained by combining them.
When the amino acid sequence is inserted, deleted or substituted as described above, the position of the insertion, deletion or substitution is not particularly limited.
[0010]
In the protein in the present specification, the left end is the N-terminus (amino terminus) and the right end is the C-terminus (carboxyl terminus) according to the convention of peptide labeling. The protein used in the present invention, including the protein containing the amino acid sequence represented by SEQ ID NO: 1, has a carboxyl group (-COOH) and a carboxylate (-COO) at the C-terminus. ⁻ ), Amide (-CONH ₂ )) Or an ester (—COOR).
Here, as R in the ester, for example, C, such as methyl, ethyl, n-propyl, isopropyl, n-butyl, etc. _1-6 Alkyl groups such as C, cyclopentyl, cyclohexyl, etc. _3-8 Cycloalkyl groups such as phenyl, α-naphthyl and the like; _6-12 Aryl groups, for example phenyl-C such as benzyl, phenethyl, etc. _1-2 An alkyl group or α-naphthyl-C such as α-naphthylmethyl _1-2 C such as an alkyl group _7-14 An aralkyl group, a pivaloyloxymethyl group and the like are used.
When the protein used in the present invention has a carboxyl group (or carboxylate) other than the C-terminus, the protein used in the present invention includes those in which the carboxyl group is amidated or esterified. As the ester in this case, for example, the above-mentioned C-terminal ester and the like are used.
Furthermore, in the protein used in the present invention, the amino group of the N-terminal amino acid residue (eg, a methionine residue) has a protecting group (for example, a formyl group, an acetyl group or the like). _1-6 C such as alkanoyl _1-6 Acyl group), N-terminal glutamine residue generated by cleavage in vivo, pyroglutamine oxidation, substituent on the side chain of amino acid in the molecule (eg, -OH, -SH , An amino group, an imidazole group, an indole group, a guanidino group, etc.) are suitable protecting groups (for example, formyl group, acetyl group, etc.). _1-6 C such as alkanoyl group _1-6 (Eg, an acyl group), or a complex protein such as a so-called glycoprotein to which a sugar chain is bound.
Specific examples of the protein used in the present invention include, for example, a protein containing the amino acid sequence represented by SEQ ID NO: 1, a protein containing the amino acid sequence represented by SEQ ID NO: 3, and the like.
[0011]
The partial peptide of the protein used in the present invention is a partial peptide of the protein used in the present invention described above, and is preferably any peptide having the same properties as the protein used in the present invention described above. It may be something. Specifically, for the purpose of preparing the antibody of the present invention described below, a peptide having the amino acid sequence at positions 30 to 48 in the amino acid sequence represented by SEQ ID NO: 1, the amino acid represented by SEQ ID NO: 3 Peptides having the amino acid sequence at positions 30 to 48 in the sequence are exemplified. For example, it has at least 20 or more, preferably 50 or more, more preferably 70 or more, more preferably 100 or more, and most preferably 200 or more amino acid sequences among the constituent amino acid sequences of the protein used in the present invention. Peptides and the like are used.
In the partial peptide used in the present invention, one or more (preferably about 1 to 10, more preferably a number (1 to 5)) amino acids in the amino acid sequence are deleted, or One or more (preferably about 1 to 20, more preferably about 1 to 10, and still more preferably, about 1 to 5) amino acids are added to the amino acid sequence, or the amino acid One or more (preferably about 1 to 20, more preferably about 1 to 10, and still more preferably, about 1 to 5) amino acids are inserted into the sequence, or One or more (preferably about 1 to 10, more preferably several, and still more preferably about 1 to 5) amino acids may be substituted with another amino acid.
[0012]
The partial peptide used in the present invention has a carboxyl group (—COOH) and a carboxylate (—COO) at the C-terminus. ⁻ ), Amide (-CONH ₂ )) Or an ester (—COOR).
Further, the partial peptides used in the present invention include those having a carboxyl group (or carboxylate) in addition to the C-terminus and the N-terminal amino acid residues (eg, , A methionine residue) in which the amino group is protected with a protecting group, a glutamine residue generated by cleavage of the N-terminal side in vivo and pyroglutamine oxidation, a substituent on the side chain of the amino acid in the molecule is Also included are those protected with an appropriate protecting group, and complex peptides such as so-called glycopeptides to which sugar chains are bound.
The partial peptide used in the present invention can also be used as an antigen for preparing an antibody.
[0013]
As the salt of the protein or partial peptide used in the present invention, salts with physiologically acceptable acids (eg, inorganic acids, organic acids) and bases (eg, alkali metal salts) are used. Are preferred. Such salts include, for example, salts with inorganic acids (eg, hydrochloric acid, phosphoric acid, hydrobromic acid, sulfuric acid) or organic acids (eg, acetic acid, formic acid, propionic acid, fumaric acid, maleic acid, succinic acid) Acids, tartaric acid, citric acid, malic acid, oxalic acid, benzoic acid, methanesulfonic acid, benzenesulfonic acid) and the like are used.
The protein or its partial peptide or its salt used in the present invention can be produced from the above-mentioned human or warm-blooded animal cells or tissues by a known method for purifying a protein or contains a DNA encoding the protein. It can also be produced by culturing a transformant. Further, it can be produced according to the peptide synthesis method described later.
When producing from human or mammalian tissues or cells, the homogenized human or mammalian tissues or cells are extracted with an acid or the like, and the extract is subjected to chromatography such as reverse phase chromatography or ion exchange chromatography. Can be purified and isolated.
[0014]
For the synthesis of the protein or partial peptide or a salt thereof, or an amide thereof used in the present invention, a commercially available resin for protein synthesis can be generally used. Examples of such a resin include chloromethyl resin, hydroxymethyl resin, benzhydrylamine resin, aminomethyl resin, 4-benzyloxybenzyl alcohol resin, 4-methylbenzhydrylamine resin, PAM resin, and 4-hydroxymethylmethyl. Phenylacetamidomethyl resin, polyacrylamide resin, 4- (2 ′, 4′-dimethoxyphenyl-hydroxymethyl) phenoxy resin, 4- (2 ′, 4′-dimethoxyphenyl-Fmocaminoethyl) phenoxy resin, and the like. it can. Using such a resin, an amino acid having an α-amino group and a side chain functional group appropriately protected is condensed on the resin in accordance with the sequence of the target protein according to various known condensation methods. At the end of the reaction, the protein or partial peptide is cleaved from the resin, and at the same time, various protecting groups are removed.In addition, an intramolecular disulfide bond formation reaction is performed in a highly diluted solution to obtain the target protein or partial peptide or an amide thereof. I do.
For the condensation of the above protected amino acids, various activating reagents that can be used for protein synthesis can be used, and carbodiimides are particularly preferable. As the carbodiimides, DCC, N, N′-diisopropylcarbodiimide, N-ethyl-N ′-(3-dimethylaminoprolyl) carbodiimide and the like are used. For activation by these, the protected amino acid was directly added to the resin together with a racemization inhibitor additive (for example, HOBt, HOOBt), or the protected amino acid was previously activated as a symmetric acid anhydride or HOBt ester or HOOBt ester. Later it can be added to the resin.
[0015]
The solvent used for activating the protected amino acid or condensing with the resin can be appropriately selected from solvents known to be usable for the protein condensation reaction. For example, acid amides such as N, N-dimethylformamide, N, N-dimethylacetamide, N-methylpyrrolidone, halogenated hydrocarbons such as methylene chloride and chloroform, alcohols such as trifluoroethanol, and dimethyl sulfoxide. Sulfoxides, ethers such as pyridine, dioxane, and tetrahydrofuran, nitriles such as acetonitrile and propionitrile, esters such as methyl acetate and ethyl acetate, and appropriate mixtures thereof are used. The reaction temperature is appropriately selected from a range known to be usable for a protein bond formation reaction, and is usually appropriately selected from a range of about -20 ° C to 50 ° C. The activated amino acid derivative is usually used in a 1.5 to 4-fold excess. As a result of the test using the ninhydrin reaction, when the condensation is insufficient, sufficient condensation can be performed by repeating the condensation reaction without removing the protecting group. When sufficient condensation cannot be obtained even by repeating the reaction, unreacted amino acids can be acetylated using acetic anhydride or acetylimidazole to prevent the subsequent reaction from being affected.
[0016]
Examples of the protecting group for the amino group of the starting material include Z, Boc, t-pentyloxycarbonyl, isobornyloxycarbonyl, 4-methoxybenzyloxycarbonyl, Cl-Z, Br-Z, adamantyloxycarbonyl, trifluoroacetyl , Phthaloyl, formyl, 2-nitrophenylsulfenyl, diphenylphosphinothioyl, Fmoc and the like.
The carboxyl group may be, for example, a linear, branched or cyclic alkyl ester such as an alkyl esterified ester (eg, methyl, ethyl, propyl, butyl, t-butyl, cyclopentyl, cyclohexyl, cycloheptyl, cyclooctyl, 2-adamantyl). ), Aralkyl esterification (eg, benzyl ester, 4-nitrobenzyl ester, 4-methoxybenzyl ester, 4-chlorobenzyl ester, benzhydryl esterification), phenacyl esterification, benzyloxycarbonylhydrazide, t-butoxy It can be protected by carbonyl hydrazide, trityl hydrazide and the like.
The hydroxyl group of serine can be protected, for example, by esterification or etherification. Suitable groups for this esterification include, for example, lower (C _1-6 A) Groups derived from carbonic acid such as an aroyl group such as an alkanoyl group and a benzoyl group, and a benzyloxycarbonyl group and an ethoxycarbonyl group. Examples of the group suitable for etherification include a benzyl group, a tetrahydropyranyl group, and a t-butyl group.
Examples of the protecting group for the phenolic hydroxyl group of tyrosine include Bzl, Cl ₂ -Bzl, 2-nitrobenzyl, Br-Z, t-butyl and the like are used.
As the imidazole protecting group for histidine, for example, Tos, 4-methoxy-2,3,6-trimethylbenzenesulfonyl, DNP, benzyloxymethyl, Bum, Boc, Trt, Fmoc and the like are used.
[0017]
Examples of the activated carboxyl group of the raw material include, for example, a corresponding acid anhydride, azide, active ester [alcohol (eg, pentachlorophenol, 2,4,5-trichlorophenol, 2,4-dinitrophenol, Cyanomethyl alcohol, paranitrophenol, HONB, N-hydroxysuccinimide, N-hydroxyphthalimide, and an ester with HOBt). As the activated amino group of the raw material, for example, a corresponding phosphoric amide is used.
As a method for removing (eliminating) the protecting group, for example, catalytic reduction in a hydrogen stream in the presence of a catalyst such as Pd-black or Pd-carbon, or hydrogen fluoride anhydride, methanesulfonic acid, trifluoromethane, etc. Acid treatment with dichloromethane, trifluoroacetic acid or a mixture thereof, base treatment with diisopropylethylamine, triethylamine, piperidine, piperazine, etc., reduction with sodium in liquid ammonia, and the like are also used. The elimination reaction by the above acid treatment is generally performed at a temperature of about -20 ° C to 40 ° C. In the acid treatment, for example, anisole, phenol, thioanisole, metacresol, paracresol, dimethylsulfide, 1,4 -Addition of a cation scavenger such as butanedithiol, 1,2-ethanedithiol and the like is effective. Further, the 2,4-dinitrophenyl group used as an imidazole protecting group of histidine is removed by thiophenol treatment, and the formyl group used as an indole protecting group of tryptophan is the above 1,2-ethanedithiol, 1,4-butane. In addition to deprotection by acid treatment in the presence of dithiol or the like, it is also removed by alkali treatment with dilute sodium hydroxide solution, dilute ammonia or the like.
[0018]
The protection of the functional group that should not be involved in the reaction of the raw materials, the protective group, the elimination of the protective group, the activation of the functional group involved in the reaction, and the like can be appropriately selected from known groups or known means.
As another method for obtaining an amide form of a protein or a partial peptide, for example, after amidating and protecting the α-carboxyl group of the carboxy terminal amino acid, a peptide (protein) chain is added to the amino group side to a desired chain length. After the elongation, a protein or partial peptide from which only the protecting group for the N-terminal α-amino group of the peptide chain has been removed and a protein or partial peptide from which only the protecting group for the C-terminal carboxyl group has been removed, and these are produced. The protein or peptide is condensed in a mixed solvent as described above. Details of the condensation reaction are the same as described above. After purifying the protected protein or peptide obtained by the condensation, all the protecting groups are removed by the above-mentioned method to obtain a desired crude protein or peptide. This crude protein or peptide is purified by various known purification means, and the main fraction is lyophilized to obtain an amide of the desired protein or peptide.
In order to obtain an ester of a protein or peptide, for example, after condensing the α-carboxyl group of the carboxy terminal amino acid with a desired alcohol to form an amino acid ester, the desired protein or An ester of the peptide can be obtained.
[0019]
The partial peptide or a salt thereof used in the present invention can be produced according to a peptide synthesis method known per se, or by cleaving the protein used in the present invention with an appropriate peptidase. As a method for synthesizing a peptide, for example, any of a solid phase synthesis method and a liquid phase synthesis method may be used. That is, the partial peptide or amino acid that can constitute the partial peptide used in the present invention is condensed with the remaining portion, and when the product has a protecting group, the protecting group is eliminated to produce the target peptide. it can. Known condensation methods and elimination of protecting groups include, for example, the methods described in the following (1) to (5).
{1} M. Bodanszky and M.A. A. Ondetti, Peptide Synthesis, Interscience Publishers, New York (1966)
(2) Schroeder and Luebke, The Peptide, Academic Press, New York (1965)
(3) Nobuo Izumiya et al., Fundamentals and experiments of peptide synthesis, Maruzen Co., Ltd. (1975)
(4) Haruaki Yajima and Shunpei Sakakibara, Biochemistry Laboratory Course 1, Protein Chemistry IV, 205, (1977)
5) Supervision of Haruaki Yajima, Development of Continuing Drugs, Volume 14, Peptide Synthesis, Hirokawa Shoten
After the reaction, the partial peptide used in the present invention can be purified and isolated by a combination of ordinary purification methods such as solvent extraction, distillation, column chromatography, liquid chromatography, and recrystallization. When the partial peptide obtained by the above method is a free form, it can be converted to an appropriate salt by a known method or a method analogous thereto, and conversely, when the partial peptide is obtained as a salt, a known method or analogous method It can be converted into a free form or another salt by a method.
[0020]
The polynucleotide encoding the protein used in the present invention may be any polynucleotide as long as it contains the above-described nucleotide sequence encoding the protein used in the present invention. Preferably it is DNA. The DNA may be any of genomic DNA, genomic DNA library, cDNA derived from the above-described cells / tissues, cDNA library derived from the aforementioned cells / tissues, and synthetic DNA.
The vector used for the library may be any of bacteriophage, plasmid, cosmid, phagemid and the like. Alternatively, amplification can be carried out directly by Reverse Transcriptase Polymerase Chain Reaction (hereinafter abbreviated as RT-PCR method) using a total RNA or mRNA fraction prepared from the above-mentioned cells / tissues.
The DNA encoding the protein used in the present invention includes, for example, a DNA containing the nucleotide sequence represented by SEQ ID NO: 2 or a nucleotide sequence hybridized with the nucleotide sequence represented by SEQ ID NO: 2 under high stringency conditions. Any DNA may be used as long as it contains a soybean base sequence and encodes a protein having substantially the same properties as the protein containing the amino acid sequence represented by SEQ ID NO: 1.
[0021]
Examples of the DNA that can hybridize with the base sequence represented by SEQ ID NO: 2 under high stringency conditions include, for example, about 50% or more, preferably about 60% or more with the base sequence represented by SEQ ID NO: 2. More preferably, a DNA containing a base sequence having a homology of about 70% or more, more preferably about 80% or more, particularly preferably about 90% or more, and most preferably about 95% or more is used. For example, a DNA containing the base sequence represented by SEQ ID NO: 4 and the like can be mentioned.
The homology of the nucleotide sequences was determined using the homology calculation algorithm NCBI BLAST (National Center for Biotechnology Information Basic Local Alignment Search Tool) under the following conditions (expected value = 10; gap allowed; filtering = ON; match score = 1; Mismatch score = −3).
Hybridization can be performed according to a method known per se or a method analogous thereto, for example, the method described in Molecular Cloning 2nd (J. Sambrook et al., Cold Spring Harbor Lab. Press, 1989). When a commercially available library is used, it can be performed according to the method described in the attached instruction manual. More preferably, it can be performed under high stringent conditions.
The high stringent conditions are, for example, conditions in which the sodium concentration is about 19 to 40 mM, preferably about 19 to 20 mM, and the temperature is about 50 to 70 ° C, preferably about 60 to 65 ° C. In particular, the case where the sodium concentration is about 19 mM and the temperature is about 65 ° C. is most preferable.
More specifically, as the DNA encoding the protein containing the amino acid sequence represented by SEQ ID NO: 1, a DNA containing the base sequence represented by SEQ ID NO: 2 or the like is represented by SEQ ID NO: 3. As a DNA encoding a protein containing the amino acid sequence represented by SEQ ID NO: 4, a DNA containing the base sequence represented by SEQ ID NO: 4 or the like is used.
[0022]
The polynucleotide (eg, DNA) encoding the partial peptide used in the present invention may be any polynucleotide containing the above-described nucleotide sequence encoding the partial peptide used in the present invention. Further, any of genomic DNA, genomic DNA library, cDNA derived from the above-mentioned cells / tissues, cDNA library derived from the aforementioned cells / tissues, and synthetic DNA may be used.
As the DNA encoding the partial peptide used in the present invention, for example, a DNA containing a part of the DNA containing the base sequence represented by SEQ ID NO: 2 or a DNA containing a part of the base sequence represented by SEQ ID NO: 2 DNAs containing a base sequence that hybridizes under stringent conditions and containing a part of a DNA encoding a protein having substantially the same activity as the protein of the present invention are used. The DNA hybridizable to the base sequence represented by SEQ ID NO: 2 has the same significance as described above.
The same hybridization method and high stringency conditions as described above are used.
[0023]
Means for cloning a DNA that completely encodes the protein or partial peptide used in the present invention (hereinafter, in the description of the cloning and expression of the DNA encoding the same, these may be simply abbreviated as the protein of the present invention) Amplification by a PCR method using a synthetic DNA primer containing a part of the nucleotide sequence encoding the protein of the present invention, or the DNA incorporated into an appropriate vector is used to obtain a partial or whole region of the protein of the present invention. Screening can be carried out by hybridization with a DNA fragment to be coded or labeled with a synthetic DNA. Hybridization can be performed, for example, according to the method described in Molecular Cloning 2nd (J. Sambrook et al., Cold Spring Harbor Lab. Press, 1989). When a commercially available library is used, it can be performed according to the method described in the attached instruction manual.
Conversion of the base sequence of DNA can be performed by PCR, a known kit, for example, Mutan. ^TM -Super Express Km (Takara Shuzo Co., Ltd.), Mutan ^TM Using -K (Takara Shuzo Co., Ltd.) or the like, it can be carried out according to a method known per se such as the ODA-LA PCR method, the Gapped Duplex method, the Kunkel method, or a method similar thereto.
The DNA encoding the cloned protein can be used as it is or as desired, after digestion with a restriction enzyme or addition of a linker, if desired. The DNA may have ATG as a translation initiation codon at the 5 'end and TAA, TGA or TAG as a translation termination codon at the 3' end. These translation initiation codon and translation termination codon can also be added using an appropriate synthetic DNA adapter.
The expression vector for the protein of the present invention includes, for example, (a) cutting out a DNA fragment of interest from DNA encoding the protein of the present invention, and (b) ligating the DNA fragment downstream of a promoter in an appropriate expression vector. It can be manufactured by the following.
[0024]
Examples of the vector include plasmids derived from Escherichia coli (eg, pBR322, pBR325, pUC12, pUC13), plasmids derived from Bacillus subtilis (eg, pUB110, pTP5, pC194), plasmids derived from yeast (eg, pSH19, pSH15), λ phage and the like. In addition to animal viruses such as bacteriophage, retrovirus, vaccinia virus, and baculovirus, pA1-11, pXT1, pRc / CMV, pRc / RSV, pcDNAI / Neo, and the like are used.
The promoter used in the present invention may be any promoter as long as it is appropriate for the host used for gene expression. For example, when an animal cell is used as a host, SRα promoter, SV40 promoter, LTR promoter, CMV promoter, HSV-TK promoter and the like can be mentioned.
Of these, it is preferable to use a CMV (cytomegalovirus) promoter, SRα promoter, or the like. When the host is Escherichia, trp promoter, lac promoter, recA promoter, λP _L Promoter, lpp promoter, T7 promoter, etc., when the host is Bacillus, SPO1 promoter, SPO2 promoter, penP promoter, etc., and when the host is yeast, PHO5 promoter, PGK promoter, GAP promoter, ADH promoter, etc. Is preferred. When the host is an insect cell, a polyhedrin promoter, a P10 promoter and the like are preferable.
[0025]
In addition to the above, an expression vector containing an enhancer, a splicing signal, a polyA addition signal, a selection marker, an SV40 replication origin (hereinafter sometimes abbreviated as SV40 ori), and the like may be used, if desired. it can. Examples of the selectable marker include a dihydrofolate reductase (hereinafter sometimes abbreviated as dhfr) gene [methotrexate (MTX) resistance] and an ampicillin resistance gene (hereinafter Amp). ^r Neomycin resistance gene (hereinafter Neo). ^r G418 resistance). In particular, when the dhfr gene is used as a selection marker using Chinese hamster cells deficient in dhfr gene, the target gene can be selected using a thymidine-free medium.
If necessary, a signal sequence suitable for the host is added to the N-terminal side of the protein of the present invention. When the host is a genus Escherichia, a PhoA signal sequence, an OmpA signal sequence, or the like is used. When the host is a Bacillus genus, an α-amylase signal sequence, a subtilisin signal sequence, or the like is used. In some cases, MFα signal sequence, SUC2 signal sequence, etc., and when the host is an animal cell, insulin signal sequence, α-interferon signal sequence, antibody molecule, signal sequence, etc. can be used.
A transformant can be produced using the vector containing the DNA encoding the protein of the present invention thus constructed.
[0026]
As the host, for example, Escherichia, Bacillus, yeast, insect cells, insects, animal cells and the like are used.
Specific examples of the genus Escherichia include, for example, Escherichia coli K12.DH1 [Proc. Natl. Acad. Sci. USA, 60, 160 (1968)], JM103 [Nucleic Acids Research, 9, 309 (1981)], JA221 [Journal of Molecular Biology, 120, 517 (1978)], HB101 [Journalolology]. , 459 (1969)], C600 [Genetics, 39, 440 (1954)] and the like.
As the Bacillus bacterium, for example, Bacillus subtilis MI114 [Gene, 24, 255 (1983)], 207-21 [Journal of Biochemistry, 95, 87 (1984)] and the like are used.
Examples of yeast include Saccharomyces cerevisiae AH22 and AH22R. ⁻ , NA87-11A, DKD-5D, 20B-12, Schizosaccharomyces pombe NCYC1913, NCYC2036, Pichia pastoris KM71 and the like.
[0027]
When the virus is AcNPV, for example, when the virus is AcNPV, a cell line derived from a larva of night roth moth (Spodoptera frugiperda cell; Sf cell), MG1 cell derived from the midgut of Trichoplusia ni, and Hig derived from Trichoplusia ni egg. ^TM Cells, cells derived from Mamestra brassicae, cells derived from Estigmena acrea, and the like are used. When the virus is BmNPV, a silkworm-derived cell line (Bombyx mori N cell; BmN cell) or the like is used. As the Sf cells, for example, Sf9 cells (ATCC CRL 1711), Sf21 cells (above, Vaughn, JL, et al., In Vivo, 13, 213-217, (1977)) and the like are used.
As the insect, for example, a silkworm larva is used [Maeda et al., Nature, 315, 592 (1985)].
Examples of animal cells include monkey cells COS-7, Vero, Chinese hamster cells CHO (hereinafter abbreviated as CHO cells), dhfr gene-deficient Chinese hamster cells CHO (hereinafter CHO (dhfr). ⁻ ) Cells), mouse L cells, mouse AtT-20, mouse myeloma cells, mouse ATDC5 cells, rat GH3, human FL cells, and the like.
For transformation of Escherichia, for example, Proc. Natl. Acad. Sci. USA, 69, 2110 (1972) and Gene, 17, 107 (1982).
[0028]
Bacillus spp. Can be transformed, for example, according to the method described in Molecular & General Genetics, vol. 168, 111 (1979).
To transform yeast, see, for example, Methods in Enzymology, Vol. 194, 182-187 (1991), Proc. Natl. Acad. Sci. USA, Vol. 75, 1929 (1978).
Insect cells or insects can be transformed, for example, according to the method described in Bio / Technology, 6, 47-55 (1988).
To transform animal cells, for example, see Cell Engineering Separate Volume 8, New Cell Engineering Experiment Protocol. 263-267 (1995) (published by Shujunsha) and Virology, Vol. 52, 456 (1973).
Thus, a transformant transformed with the expression vector containing the DNA encoding the protein can be obtained.
When culturing a transformant whose host is a genus Escherichia or Bacillus, a liquid medium is suitable as a medium used for the culturing, and a carbon source necessary for growth of the transformant is used therein. Nitrogen sources, inorganic substances, etc. are included. As a carbon source, for example, glucose, dextrin, soluble starch, sucrose, etc., as a nitrogen source, for example, ammonium salts, nitrates, corn steep liquor, peptone, casein, meat extract, soybean meal, potato extract and the like Examples of the inorganic or organic substance and the inorganic substance include calcium chloride, sodium dihydrogen phosphate, and magnesium chloride. In addition, yeast extract, vitamins, growth promoting factors and the like may be added. The pH of the medium is preferably about 5 to 8.
[0029]
As a medium for culturing the genus Escherichia, for example, an M9 medium containing glucose and casamino acid [Miller, Journal of Experiments in Molecular Genetics, 431-433, Cold Spring Harbor Laboratory, New York, New York, 1972] is preferable. If necessary, an agent such as 3β-indolylacrylic acid can be added in order to make the promoter work efficiently.
When the host is a bacterium belonging to the genus Escherichia, the cultivation is usually performed at about 15 to 43 ° C. for about 3 to 24 hours, and if necessary, aeration and stirring can be added.
When the host is a bacterium belonging to the genus Bacillus, the cultivation is usually carried out at about 30 to 40 ° C. for about 6 to 24 hours, and if necessary, aeration and stirring may be added.
When culturing a transformant in which the host is yeast, for example, Burkholder's minimum medium [Bostian, K. et al. L. Proc. Natl. Acad. Sci. USA, Vol. 77, 4505 (1980)] or an SD medium containing 0.5% casamino acid [Bitter, G. et al. A. Proc. Natl. Acad. Sci. USA, 81, 5330 (1984)]. Preferably, the pH of the medium is adjusted to about 5-8. The cultivation is usually performed at about 20 ° C. to 35 ° C. for about 24 to 72 hours, and if necessary, aeration and stirring are added.
When culturing an insect cell or a transformant whose host is an insect, the medium was immobilized as Grace's Insect Medium (Grace, TCC, Nature, 195, 788 (1962)). Those to which additives such as 10% bovine serum are appropriately added are used. The pH of the medium is preferably adjusted to about 6.2 to 6.4. The cultivation is usually performed at about 27 ° C. for about 3 to 5 days, and if necessary, aeration or stirring is added.
When culturing a transformant in which the host is an animal cell, examples of the medium include a MEM medium containing about 5 to 20% fetal bovine serum [Science, Vol. 122, 501 (1952)], a DMEM medium [Virology, 8, 396 (1959)], RPMI 1640 medium [The Journal of the American Medical Association, 199, 519 (1967)], and 199 medium [Proceeding of the Society for Biotechnology, etc., 73, etc. Is used. Preferably, the pH is between about 6 and 8. The cultivation is usually performed at about 30 to 40 ° C. for about 15 to 60 hours, and if necessary, aeration and stirring are added.
As described above, the protein of the present invention can be produced in cells, cell membranes or extracellular cells of the transformant.
[0030]
The protein of the present invention can be separated and purified from the culture by, for example, the following method.
When extracting the protein of the present invention from cultured cells or cells, the cells or cells are collected by a known method after culturing, suspended in an appropriate buffer, and subjected to sonication, lysozyme and / or freeze-thawing. After the cells or cells are destroyed by the method, a method of obtaining a crude extract of the protein by centrifugation or filtration is used as appropriate. In a buffer, a protein denaturant such as urea or guanidine hydrochloride, or Triton X-100 is used. ^TM And the like. When the protein is secreted into the culture solution, after the culture is completed, the supernatant is separated from the cells or cells by a method known per se, and the supernatant is collected.
The protein contained in the culture supernatant or extract obtained in this manner can be purified by appropriately combining known separation and purification methods. These known separation and purification methods include methods utilizing solubility such as salting out and solvent precipitation, dialysis, ultrafiltration, gel filtration, and SDS-polyacrylamide gel electrophoresis, mainly molecular weight. Using differences in charge, methods using charge differences such as ion exchange chromatography, methods using specific affinity such as affinity chromatography, and using differences in hydrophobicity such as reversed-phase high-performance liquid chromatography A method utilizing a difference between isoelectric points, such as an isoelectric focusing method, is used.
[0031]
When the protein thus obtained is obtained in a free form, it can be converted to a salt by a method known per se or a method analogous thereto, and conversely, when it is obtained as a salt, a method known per se or analogous thereto Can be converted to a free form or another salt.
The protein produced by the recombinant can be arbitrarily modified or the polypeptide can be partially removed by allowing a suitable protein modifying enzyme to act on the protein before or after purification. As the protein modifying enzyme, for example, trypsin, chymotrypsin, arginyl endopeptidase, protein kinase, glycosidase and the like are used.
The presence of the protein of the present invention thus produced can be measured by an enzyme immunoassay using a specific antibody, Western blotting, or the like.
[0032]
The antibody against the protein or partial peptide or a salt thereof used in the present invention may be any of a polyclonal antibody and a monoclonal antibody as long as it can recognize the protein or partial peptide or a salt thereof used in the present invention.
Antibodies against the protein or partial peptide used in the present invention or a salt thereof (hereinafter sometimes simply referred to as the protein of the present invention in the description of the antibody) use the protein of the present invention as an antigen and are known per se. Can be produced according to the antibody or antiserum production method described in
[Preparation of monoclonal antibody]
(A) Preparation of monoclonal antibody-producing cells
The protein of the present invention is administered to a warm-blooded animal itself or together with a carrier and a diluent at a site capable of producing an antibody upon administration. Complete Freund's adjuvant or incomplete Freund's adjuvant may be administered in order to enhance the antibody-producing ability upon administration. The administration is usually performed once every 2 to 6 weeks, for a total of about 2 to 10 times. Examples of the warm-blooded animal used include monkeys, rabbits, dogs, guinea pigs, mice, rats, sheep, goats, and chickens, and mice and rats are preferably used.
When preparing monoclonal antibody-producing cells, a warm-blooded animal immunized with an antigen, for example, an individual having an antibody titer is selected from a mouse, and the spleen or lymph node is collected 2 to 5 days after the final immunization and contained in them. By fusing the antibody-producing cells thus obtained with myeloma cells of the same or different species, a monoclonal antibody-producing hybridoma can be prepared. The antibody titer in the antiserum can be measured, for example, by reacting a labeled protein described below with the antiserum, and then measuring the activity of a labeling agent bound to the antibody. The fusion operation can be performed according to a known method, for example, the method of Koehler and Milstein [Nature, 256, 495 (1975)]. Examples of the fusion promoter include polyethylene glycol (PEG) and Sendai virus, but PEG is preferably used.
[0033]
Examples of myeloma cells include myeloma cells of warm-blooded animals such as NS-1, P3U1, SP2 / 0, and AP-1, but P3U1 is preferably used. The preferred ratio between the number of antibody-producing cells (spleen cells) and the number of myeloma cells used is about 1: 1 to 20: 1, and PEG (preferably PEG1000 to PEG6000) is added at a concentration of about 10 to 80%. By incubating at 20 to 40 ° C, preferably 30 to 37 ° C for 1 to 10 minutes, cell fusion can be carried out efficiently. Various methods can be used to screen for monoclonal antibody-producing hybridomas. For example, a hybridoma culture supernatant is added to a solid phase (eg, a microplate) on which a protein antigen is directly or adsorbed together with a carrier, and then radioactive substances or A method for detecting a monoclonal antibody bound to a solid phase by adding an anti-immunoglobulin antibody labeled with an enzyme or the like (an anti-mouse immunoglobulin antibody is used when cells used for cell fusion are mice) or protein A; A method in which a hybridoma culture supernatant is added to a solid phase to which globulin antibodies or protein A is adsorbed, a protein labeled with a radioactive substance, an enzyme, or the like is added, and a monoclonal antibody bound to the solid phase is detected.
Selection of the monoclonal antibody can be performed according to a method known per se or a method analogous thereto. Usually, it can be performed in a medium for animal cells supplemented with HAT (hypoxanthine, aminopterin, thymidine). As a selection and breeding medium, any medium can be used as long as a hybridoma can grow. For example, RPMI 1640 medium containing 1 to 20%, preferably 10 to 20% fetal bovine serum, GIT medium containing 1 to 10% fetal bovine serum (Wako Pure Chemical Industries, Ltd.) or serum-free for hybridoma culture A medium (SFM-101, Nissui Pharmaceutical Co., Ltd.) or the like can be used. The culturing temperature is usually 20 to 40 ° C, preferably about 37 ° C. The culture time is usually 5 days to 3 weeks, preferably 1 week to 2 weeks. The culture can be usually performed under 5% carbon dioxide gas. The antibody titer of the hybridoma culture supernatant can be measured in the same manner as the measurement of the antibody titer in the antiserum described above.
[0034]
(B) Purification of monoclonal antibody
The monoclonal antibody can be separated and purified by a method known per se, for example, an immunoglobulin separation and purification method [eg, salting out method, alcohol precipitation method, isoelectric point precipitation method, electrophoresis method, ion exchanger (eg, DEAE)] Adsorption-desorption method, ultracentrifugation method, gel filtration method, antigen-binding solid phase or specific purification method of collecting antibody only with an active adsorbent such as protein A or protein G and dissociating the bond to obtain the antibody] Can be.
(Preparation of polyclonal antibody)
The polyclonal antibody of the present invention can be produced according to a method known per se or a method analogous thereto. For example, a immunizing antigen (protein antigen) itself or a complex thereof with a carrier protein is formed, and a warm-blooded animal is immunized in the same manner as in the above-described method for producing a monoclonal antibody. It can be produced by collecting a substance and separating and purifying the antibody.
Regarding the complex of an immunizing antigen and a carrier protein used to immunize a warm-blooded animal, the type of carrier protein and the mixing ratio of the carrier and the hapten are such that the antibody is efficiently cross-linked to the hapten immunized by crosslinking the carrier. If possible, any material may be cross-linked at any ratio. For example, bovine serum albumin, bovine thyroglobulin, hemocyanin, etc. are used in a weight ratio of about 0.1 to 20, preferably about 1 to 20, relative to hapten 1. A method of coupling at a rate of ~ 5 is used. Various coupling agents can be used for coupling the hapten and the carrier, and glutaraldehyde, carbodiimide, a maleimide active ester, an active ester reagent containing a thiol group or a dithioviridyl group, or the like is used.
The condensation product is administered to a warm-blooded animal itself or together with a carrier or diluent at a site where antibody production is possible. Complete Freund's adjuvant or incomplete Freund's adjuvant may be administered in order to enhance the antibody-producing ability upon administration. The administration is usually performed once every about 2 to 6 weeks, about 3 to 10 times in total.
The polyclonal antibody can be collected from the blood, ascites, or the like, preferably from the blood of a warm-blooded animal immunized by the above method.
The measurement of the polyclonal antibody titer in the antiserum can be performed in the same manner as the measurement of the antibody titer in the antiserum described above. The separation and purification of the polyclonal antibody can be performed according to the same immunoglobulin separation and purification method as the above-mentioned separation and purification of the monoclonal antibody.
[0035]
The nucleotide sequence of a polynucleotide encoding a protein or a partial peptide used in the present invention (eg, DNA (hereinafter, these DNAs may be abbreviated to DNA of the present invention in the description of antisense polynucleotide)) The antisense polynucleotide having a complementary or substantially complementary base sequence or a part thereof includes a base sequence complementary to or substantially complementary to the base sequence of the DNA of the present invention or a part thereof. Any antisense polynucleotide may be used as long as it has a portion and has an action of suppressing the expression of the DNA, but antisense DNA is preferable.
The nucleotide sequence substantially complementary to the DNA of the present invention is, for example, about 70% of the total nucleotide sequence or a partial nucleotide sequence of the nucleotide sequence complementary to the DNA of the present invention (that is, the complementary strand of the DNA of the present invention). % Or more, preferably about 80% or more, more preferably about 90% or more, most preferably about 95% or more. In particular, in the case of an antisense polynucleotide directed to translation inhibition, of the entire base sequence of the complementary strand of the DNA of the present invention, the base sequence of the portion encoding the N-terminal site of the protein of the present invention (for example, An antisense polynucleotide having a homology of about 70% or more, preferably about 80% or more, more preferably about 90% or more, and most preferably about 95% or more with a complementary strand of a base sequence near a codon, etc. B) In the case of an antisense polynucleotide that directs RNA degradation by RNase H, it is about 70% or more, preferably about 80% or more, more preferably about 90% with the complementary strand of the entire base sequence of the DNA of the present invention including introns. As described above, most preferably, antisense polynucleotides having about 95% or more homology are suitable.
Specifically, (1) an antisense polynucleotide containing a base sequence complementary to or substantially complementary to the base sequence of DNA containing the base sequence represented by SEQ ID NO: 2, or a part thereof Preferably, for example, an antisense polynucleotide containing a nucleotide sequence complementary to the nucleotide sequence of the DNA containing the nucleotide sequence represented by SEQ ID NO: 2 or a part thereof (more preferably, an antisense polynucleotide represented by SEQ ID NO: 2 (2) a base sequence complementary to the base sequence of the DNA containing the base sequence, or (2) a base sequence of the DNA containing the base sequence represented by SEQ ID NO: 4; Antisense polynucleotide containing a specific or substantially complementary base sequence, or a portion thereof, preferably, for example, SEQ ID NO: 4 A base sequence complementary to the base sequence of the DNA containing the base sequence represented, or an antisense polynucleotide containing a part thereof (more preferably, the base sequence of the DNA containing the base sequence represented by SEQ ID NO: 4) (An antisense polynucleotide containing a nucleotide sequence complementary to or a part thereof), and the like.
The antisense polynucleotide is usually composed of about 10 to 40, preferably about 15 to 30 bases.
In order to prevent degradation by a hydrolase such as nuclease, a phosphate residue (phosphate) of each nucleotide constituting the antisense DNA may be, for example, a chemically modified phosphate residue such as phosphorothioate, methylphosphonate, or phosphorodithionate. It may be substituted. In addition, the sugar (deoxyribose) of each nucleotide may be substituted with a chemically modified sugar structure such as 2′-O-methylation, and the base portion (pyrimidine, purine) may also be chemically modified. Or any one that hybridizes to the DNA having the base sequence represented by SEQ ID NO: 2. These antisense polynucleotides can be produced using a known DNA synthesizer or the like.
[0036]
According to the present invention, an antisense polynucleotide capable of inhibiting the replication or expression of the protein gene of the present invention is cloned or designed based on the nucleotide sequence information of DNA encoding the determined protein, and synthesized. Can. Such nucleotides (nucleic acids) can hybridize with the RNA of the protein gene of the present invention and inhibit the synthesis or function of the RNA, or through interaction with the protein-related RNA of the present invention. The expression of the protein gene of the present invention can be regulated and controlled. Polynucleotides that are complementary to a selected sequence of the protein-associated RNA of the present invention, and that can specifically hybridize with the protein-associated RNA of the present invention, can be used in vivo and in vitro to produce the protein gene of the present invention. It is useful for regulating and controlling the expression of, and also useful for treating or diagnosing diseases and the like. The term “corresponding” means having homology or being complementary to a specific sequence of nucleotides, base sequences or nucleic acids including genes. "Corresponding" between a nucleotide, base sequence or nucleic acid and a peptide (protein) usually refers to the amino acid of the peptide (protein) as directed by the nucleotide (nucleic acid) sequence or its complement. . 5 'end hairpin loop of protein gene, 5' end 6-base pair repeat, 5 'end untranslated region, polypeptide translation start codon, protein coding region, ORF translation stop codon, 3' end untranslated region, 3 ' The terminal palindrome region and the 3'-end hairpin loop may be selected as preferred regions of interest, but any region within the protein gene may be selected as a target.
The relationship between the target nucleic acid and a polynucleotide complementary to at least a part of the target region can be said to be "antisense" if the relationship between the target nucleic acid and a polynucleotide capable of hybridizing with the target is. Antisense polynucleotides include polynucleotides containing 2-deoxy-D-ribose, polynucleotides containing D-ribose, other types of polynucleotides that are N-glycosides of purine or pyrimidine bases, or Other polymers having non-nucleotide backbones (eg, commercially available protein nucleic acids and synthetic sequence-specific nucleic acid polymers) or other polymers containing special bonds, provided that the polymer is a base such as found in DNA or RNA And nucleotides having a configuration permitting the attachment of a base). They can be double-stranded DNA, single-stranded DNA, double-stranded RNA, single-stranded RNA, and also DNA: RNA hybrids, and can be unmodified polynucleotides (or unmodified oligonucleotides), or even known. Such as labeled, capped, methylated, one or more naturally-occurring nucleotides replaced by analogs, intramolecular nucleotides Modified, eg, those having an uncharged bond (eg, methylphosphonate, phosphotriester, phosphoramidate, carbamate, etc.), charged or sulfur-containing bonds (eg, phosphorothioate, phosphorodithioate, etc.) ), Such as proteins (nucleases, nuclease inhibitors, Those having side-chain groups such as syn, antibody, signal peptide, poly-L-lysine, etc. and sugars (eg, monosaccharide), those having intercalating compounds (eg, acridine, psoralen) Containing chelating compounds (eg, metals, radioactive metals, boron, oxidizing metals, etc.), those containing alkylating agents, those having modified bonds (eg, α-anomeric nucleic acids) Etc.). Here, "nucleoside", "nucleotide", and "nucleic acid" may include not only those containing purine and pyrimidine bases but also those having other modified heterocyclic bases. Such modifications may include methylated purines and pyrimidines, acylated purines and pyrimidines, or other heterocycles. Modified nucleotides and modified nucleotides may also be modified at the sugar moiety, e.g., where one or more hydroxyl groups have been replaced by halogens, aliphatic groups, etc., or by functional groups such as ethers, amines, etc. It may have been converted.
The antisense polynucleotide of the present invention is RNA, DNA, or a modified nucleic acid (RNA, DNA). Specific examples of the modified nucleic acid include, but are not limited to, sulfur derivatives and thiophosphate derivatives of nucleic acids, and those that are resistant to degradation of polynucleoside amides and oligonucleoside amides. The antisense nucleic acid of the present invention can be preferably designed according to the following policy. That is, to make the antisense nucleic acid more stable in the cell, to make the antisense nucleic acid more cell permeable, to have a greater affinity for the target sense strand, and to be more toxic if it is toxic. Minimize the toxicity of sense nucleic acids.
Thus, many modifications are known in the art, for example, Kawakami et al. , Pharm Tech Japan, Vol. 8, pp. 247, 1992; Vol. 8, pp. 395, 1992; T. Crooke et al. ed. , Antisense Research and Applications, CRC Press, 1993.
The antisense nucleic acid of the present invention may contain altered or modified sugars, bases or bonds, may be provided in a special form such as liposomes or microspheres, may be applied by gene therapy, It could be provided in an added form. Thus, in the form of addition, polycations such as polylysine which acts to neutralize the charge of the phosphate skeleton, lipids which enhance the interaction with the cell membrane or increase the uptake of nucleic acids ( For example, hydrophobic substances such as phospholipid and cholesterol can be mentioned. Preferred lipids for addition include cholesterol and its derivatives (eg, cholesteryl chloroformate, cholic acid, etc.). These can be attached to the 3 'end or 5' end of the nucleic acid, and can be attached via a base, sugar, or intramolecular nucleoside bond. Other groups include cap groups specifically arranged at the 3 ′ end or 5 ′ end of a nucleic acid for preventing degradation by nucleases such as exonuclease and RNase. Such capping groups include, but are not limited to, hydroxyl-protecting groups known in the art, including glycols such as polyethylene glycol and tetraethylene glycol.
The inhibitory activity of the antisense nucleic acid can be examined using the transformant of the present invention, the in vivo or in vitro gene expression system of the present invention, or the in vivo or in vitro translation system of the protein of the present invention. The nucleic acid can be applied to cells by various methods known per se.
[0037]
Hereinafter, the protein or partial peptide of the present invention or a salt thereof (hereinafter, sometimes abbreviated as the protein of the present invention), a polynucleotide encoding the protein or partial peptide of the present invention (eg, DNA (hereinafter, referred to as the present invention) DNA)), an antibody against the protein or partial peptide of the present invention or a salt thereof (hereinafter, may be abbreviated as the antibody of the present invention), and an antisense polynucleotide of the DNA of the present invention (hereinafter, may be referred to as “antibody”). (May be abbreviated as the antisense polynucleotide of the present invention).
[0038]
The protein of the present invention can be used as a disease marker because its expression is increased in lungs having emphysema lesions. That is, it is useful as a marker for early diagnosis in the lung, determination of the severity of symptoms, and prediction of disease progression. Therefore, the antisense polynucleotide of the present invention, a compound or a salt thereof that inhibits the activity of the protein of the present invention, a compound or a salt thereof that inhibits the expression of the protein gene of the present invention, or a medicament containing the antibody of the present invention include, for example, , Respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergies) Rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, Glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, splenic dysfunction or chest Such as unusually accompanying immunodeficiency), can be safely used inflammatory bowel disease, as a prophylactic or therapeutic agent for allergic conjunctivitis.
[0039]
(1) Screening of drug candidate compounds for disease
Since the expression of the protein of the present invention is increased in lungs having emphysema lesions, compounds or salts thereof that regulate (preferably inhibit) the activity of the protein of the present invention include, for example, respiratory diseases [eg, chronic obstructive pulmonary disease] (Chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, Hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, Insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctiva It can be used as a prophylactic or therapeutic agent such as. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
Therefore, the protein of the present invention is useful as a reagent for screening a compound or a salt thereof that regulates (preferably, inhibits) the activity of the protein of the present invention.
That is, the present invention regulates (promotes or inhibits) (preferably inhibits) the activity (eg, cell adhesion activity, heparan sulfate proteoglycan binding activity, etc.) of the protein of the present invention characterized by using the protein of the present invention. A method for screening a compound or a salt thereof is provided.
Specifically, a comparison was made between (i) the cell adhesion activity or heparan sulfate proteoglycan binding activity of the protein of the present invention and (ii) the cell adhesion activity or heparan sulfate proteoglycan binding activity of a mixture of the protein of the present invention and a test compound. A method for screening a compound or a salt thereof that regulates (promotes or inhibits) the activity of the protein of the present invention, which is characterized in that
In the above screening method, for example, in the cases of (i) and (ii), cell adhesion activity or heparan sulfate proteoglycan binding activity and the like can be determined by a method known per se, for example, J. Am. Biol. Chem. 276 (11), 8125-8134, 2001, or the like or a method analogous thereto, and measured.
Specifically, (i) after mixing a fusion protein of the extracellular region of the protein of the present invention with an immunoglobulin Fc region and endothelial cells, a labeled (eg, enzyme-labeled) Fc region-recognizing antibody is reacted, and the substrate is reacted. Was added and the enzyme reaction was performed, and (ii) a fusion protein of the extracellular region of the protein of the present invention with the immunoglobulin Fc region and endothelial cells were mixed in the presence of the test compound, and then labeled ( For example, a compound that reacts with an Fc region-recognizing antibody, adds a substrate, and performs an enzyme reaction, measures enzyme activity, and modulates (promotes or inhibits) the activity of the protein of the present invention. Screen the salt. This reaction is performed in an appropriate buffer. Perform the washing operation as necessary. The measurement of the enzyme reaction is performed according to a known method using a microplate reader or the like.
Specifically, (i) a microplate on which heparin-BSA is immobilized and a fusion protein of the extracellular region of the protein of the present invention and the Fc region of the immunoglobulin are reacted, and then labeled (eg, enzyme Label) reacting with an antibody recognizing Fc region, adding a substrate, and performing an enzymatic reaction; (ii) a microplate on which heparin-BSA is immobilized in the presence of a test compound; and cells of the protein of the present invention. After reacting the fusion protein of the outer region with the Fc region of the immunoglobulin, the enzyme is reacted with a labeled (eg, enzyme-labeled) Fc region-recognizing antibody, a substrate is added, and an enzyme reaction is performed. The activity is measured respectively. This reaction is performed in an appropriate buffer. Perform the washing operation as necessary. The measurement of the enzyme reaction is performed according to a known method using a microplate reader or the like.
Examples of the extracellular region of the protein of the present invention include a peptide having the 1st to 319th sequence of the amino acid sequence represented by SEQ ID NO: 1. Fusion proteins between the extracellular region of the protein of the present invention and the immunoglobulin Fc region can be prepared by known methods, for example, as described in J. Am. Biol. Chem. 276 (11), 8125-8134, 2001 or a method analogous thereto. As the endothelial cells, for example, vascular endothelial cells and the like are used.
As the above-mentioned protein of the present invention, those produced by culturing cells capable of producing the protein of the present invention and the like are used. As a cell having the ability to produce the protein of the present invention, for example, a host (transformant) transformed with a vector containing the DNA encoding the protein of the present invention described above is used. As a host, for example, animal cells such as COS7 cells, CHO cells, and HEK293 cells are preferably used. For the screening, for example, a transformant in which the protein of the present invention is expressed on a cell membrane by culturing by the method described above is preferably used. The method for culturing cells capable of expressing the protein of the present invention is the same as the above-described method for culturing the transformant of the present invention.
Test compounds include, for example, peptides, proteins, non-peptidic compounds, synthetic compounds, fermentation products, cell extracts, plant extracts, animal tissue extracts, and the like.
For example, the cell adhesion activity or heparan sulfate proteoglycan binding activity in the case (ii) is increased by about 20% or more, preferably 30% or more, more preferably about 50% or more, as compared with the case (i). When the test compound is a compound that promotes the activity of the protein of the present invention, the cell adhesion activity or heparan sulfate proteoglycan binding activity in the case (ii) is about 20% or more, preferably 20% or more, as compared with the case (i). A test compound that reduces 30% or more, more preferably about 50% or more, can be selected as a compound that inhibits the activity of the protein of the present invention.
[0040]
The compound having the activity of promoting the activity of the protein of the present invention is useful as a safe and low-toxic drug for enhancing the action of the protein of the present invention.
The compound having the activity of inhibiting the activity of the protein of the present invention is a safe and low toxic drug for suppressing the physiological activity of the protein of the present invention, for example, a respiratory disease [eg, chronic obstructive pulmonary disease (chronic bronchitis) , Emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, pollinosis, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, Atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes) , Rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with spleen dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis, etc. As useful.
Compounds or salts thereof obtained using the screening method or screening kit of the present invention include, for example, peptides, proteins, non-peptidic compounds, synthetic compounds, fermentation products, cell extracts, plant extracts, animal tissue extracts And compounds selected from plasma and the like. As the salt of the compound, those similar to the aforementioned salts of the peptide of the present invention are used.
[0041]
Furthermore, since the expression of the gene encoding the protein of the present invention also increases in lung tissues having emphysema lesions, compounds or salts thereof that regulate (preferably inhibit) the expression of the gene encoding the protein of the present invention include, for example, , Respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergies) Rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, With glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, splenic dysfunction or thymic abnormalities Cormorant immunodeficiency, etc.), can be used inflammatory bowel disease, as a prophylactic or therapeutic agent for allergic conjunctivitis. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
Therefore, the polynucleotide (eg, DNA) of the present invention is useful as a reagent for screening a compound or a salt thereof that regulates (preferably, inhibits) the expression of a gene encoding the protein of the present invention.
The screening method includes (iii) culturing cells capable of producing the protein of the present invention and (iv) culturing cells capable of producing the protein used in the present invention in the presence of a test compound. A screening method characterized by performing a comparison with the case.
In the above method, in the cases (iii) and (iv), the expression level of the gene (specifically, the amount of the protein of the present invention or the amount of the mRNA encoding the protein) is measured and compared.
Examples of the test compound and cells having the ability to produce the protein of the present invention include those described above.
The protein amount is measured by a known method, for example, using an antibody recognizing the protein of the present invention, and measuring the protein present in a cell extract or the like according to a method such as Western analysis or ELISA method or a method analogous thereto. can do.
The amount of mRNA can be measured by a known method, for example, Northern hybridization using a nucleic acid containing SEQ ID NO: 2 or a part thereof as a probe, or a nucleic acid containing SEQ ID NO: 2 or a part thereof as a primer, SEQ ID NO: 4 Alternatively, it can be measured according to Northern hybridization using a nucleic acid containing a part thereof, or a PCR method using a nucleic acid containing SEQ ID NO: 4 or a part thereof as a primer or a method analogous thereto.
For example, a test compound that increases the gene expression level in the case of the above (iv) by about 20% or more, preferably 30% or more, and more preferably about 50% or more as compared with the case of the above (iii), according to the present invention As a compound that promotes the expression of the gene encoding the protein of the present invention, a test compound that inhibits about 20% or more, preferably 30% or more, more preferably about 50% or more suppresses the expression of the gene encoding the protein of the present invention. Can be selected as the compound.
[0042]
The screening kit of the present invention contains the protein or partial peptide used in the present invention or a salt thereof, or a cell capable of producing the protein or partial peptide used in the present invention.
Compounds or salts thereof obtained by using the screening method or the screening kit of the present invention are test compounds described above, for example, peptides, proteins, non-peptide compounds, synthetic compounds, fermentation products, cell extracts, plant extracts. A compound selected from animal tissue extract, plasma and the like, or a salt thereof, which regulates the activity of the protein of the present invention (eg, cell adhesion activity, heparan sulfate proteoglycan binding activity, etc.) or a salt thereof.
As the salt of the compound, those similar to the aforementioned salts of the protein of the present invention are used.
A compound or a salt thereof that regulates (preferably inhibits) the activity of the protein of the present invention and a compound or a salt thereof that regulates (preferably inhibits) the expression of a gene encoding the protein of the present invention are, for example, respiratory diseases [ Eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever) , Acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, glomerulonephritis, multiple occurrences) Immune deficiency associated with multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, splenic dysfunction or thymic abnormalities Etc.), it can be used inflammatory bowel disease, as a prophylactic or therapeutic agent for allergic conjunctivitis. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
When the compound or a salt thereof obtained by using the screening method or the screening kit of the present invention is used as the above-mentioned prophylactic / therapeutic agent, it can be formulated according to a conventional method.
[0043]
For example, compositions for oral administration include solid or liquid dosage forms, specifically tablets (including sugar-coated tablets and film-coated tablets), pills, granules, powders, and capsules (including soft capsules). Syrup, emulsion, suspension and the like. Such a composition is produced by a method known per se and contains a carrier, diluent or excipient commonly used in the field of formulation. For example, lactose, starch, sucrose, magnesium stearate and the like are used as carriers and excipients for tablets.
As a composition for parenteral administration, for example, injections, suppositories, etc. are used. Injections are intravenous injections, subcutaneous injections, intradermal injections, intramuscular injections, intravenous injections, intraarticular injections. Dosage forms such as agents. Such injections are prepared according to a method known per se, for example, by dissolving, suspending or emulsifying the antibody or a salt thereof in a sterile aqueous or oily liquid commonly used for injections. As an aqueous liquid for injection, for example, physiological saline, isotonic solution containing glucose and other auxiliary agents and the like are used, and suitable solubilizing agents, for example, alcohol (eg, ethanol), polyalcohol (eg, Propylene glycol, polyethylene glycol), nonionic surfactants (eg, polysorbate 80, HCO-50 (polyoxyethylene (50 mol) add-on of hydro- genated castor oil)) and the like may be used in combination. As the oily liquid, for example, sesame oil, soybean oil, and the like are used, and benzyl benzoate, benzyl alcohol, and the like may be used in combination as a solubilizing agent. The prepared injection is usually filled in an appropriate ampoule. Suppositories to be used for rectal administration are prepared by mixing the above antibody or a salt thereof with a conventional suppository base.
[0044]
The above-mentioned oral or parenteral pharmaceutical composition is conveniently prepared in a unit dosage form so as to be compatible with the dosage of the active ingredient. Examples of such dosage unit dosage forms include tablets, pills, capsules, injections (ampoules), suppositories, and the like. Usually, each dosage unit dosage form has a dosage of 5 to 500 mg, especially 5 to 100 mg for an injection. Other dosage forms preferably contain 10 to 250 mg of the above compound.
Each of the above-mentioned compositions may contain other active ingredients as long as the composition does not cause an undesirable interaction with the compound.
The preparations obtained in this way are safe and low toxic, for example, human or warm-blooded animals (eg, mouse, rat, rabbit, sheep, pig, cow, horse, bird, cat, dog, monkey, chimpanzee, etc.) ) Can be administered orally or parenterally.
The dose of the compound or a salt thereof varies depending on its action, target disease, administration subject, administration route and the like.For example, a compound or a salt thereof that regulates the activity of the protein of the present invention for the purpose of treating emphysema is used. When administered orally, in general, for an adult (with a body weight of 60 kg), the compound or a salt thereof is used in an amount of about 0.1 to 100 mg, preferably about 1.0 to 50 mg, more preferably about 1.0 to 50 mg per day. Administer 20 mg. When administered parenterally, the single dose of the compound or a salt thereof varies depending on the administration subject, target disease, and the like. For example, a compound or a compound that regulates the activity of the protein of the present invention for the purpose of treating emphysema or When the salt is administered to an adult (with a body weight of 60 kg) usually in the form of an injection, the compound or a salt thereof is used in an amount of about 0.01 to 30 mg, preferably about 0.1 to 20 mg, more preferably about 0.1 to 20 mg per day. Advantageously, 1 to 10 mg is administered by intravenous injection. In the case of other animals, the amount can be administered in terms of the weight per 60 kg.
[0045]
(2) Quantification of the protein of the present invention, its partial peptide or its salt
An antibody against the protein of the present invention (hereinafter sometimes abbreviated as the antibody of the present invention) can specifically recognize the protein of the present invention. It can be used for quantification by sandwich immunoassay and the like.
That is, the present invention
(I) reacting the antibody of the present invention with a test solution and a labeled protein of the present invention competitively, and measuring the ratio of the labeled protein of the present invention bound to the antibody; A method for quantifying the protein of the present invention in a test solution, and
(Ii) After reacting a test solution with the antibody of the present invention immobilized on a carrier and another labeled antibody of the present invention simultaneously or continuously, the activity of the labeling agent on the insolubilized carrier is measured. A method for quantifying the protein of the present invention in a test solution is provided.
In the quantitative method (ii), it is desirable that one antibody is an antibody that recognizes the N-terminal of the protein of the present invention and the other antibody is an antibody that reacts with the C-terminal of the protein of the present invention.
[0046]
In addition, the protein of the present invention can be quantified using a monoclonal antibody against the protein of the present invention (hereinafter sometimes referred to as the monoclonal antibody of the present invention), and can also be detected by tissue staining or the like. For these purposes, the antibody molecule itself may be used, and the F (ab ') ₂ , Fab ′ or Fab fraction may be used.
The method for quantifying the protein of the present invention using the antibody of the present invention is not particularly limited, and the antibody, antigen, or antibody-antigen complex corresponding to the amount of the antigen (eg, the amount of the protein) in the test solution is measured. Any measurement method may be used as long as the amount is detected by chemical or physical means, and the amount is calculated from a standard curve prepared using a standard solution containing a known amount of antigen. For example, nephelometry, competition method, immunometric method and sandwich method are suitably used, but it is particularly preferable to use the sandwich method described later in terms of sensitivity and specificity.
As a labeling agent used in a measuring method using a labeling substance, for example, a radioisotope, an enzyme, a fluorescent substance, a luminescent substance and the like are used. As the radioisotope, for example, [ ¹²⁵ I], [ ¹³¹ I], [ ³ H], [ ¹⁴ C] is used. As the above-mentioned enzyme, a stable enzyme having a large specific activity is preferable. For example, β-galactosidase, β-glucosidase, alkaline phosphatase, peroxidase, malate dehydrogenase and the like are used. As the fluorescent substance, for example, fluorescamine, fluorescein isothiocyanate and the like are used. As the luminescent substance, for example, luminol, a luminol derivative, luciferin, lucigenin and the like are used. Further, a biotin-avidin system can be used for binding the antibody or antigen to the labeling agent.
[0047]
For the insolubilization of an antigen or an antibody, physical adsorption may be used, or a method using a chemical bond usually used for insolubilizing and immobilizing a protein or an enzyme may be used. Examples of the carrier include insoluble polysaccharides such as agarose, dextran, and cellulose; synthetic resins such as polystyrene, polyacrylamide, and silicon; and glass.
In the sandwich method, the test solution is reacted with the insolubilized monoclonal antibody of the present invention (primary reaction), and further reacted with another labeled monoclonal antibody of the present invention (secondary reaction). By measuring the activity of the labeling agent, the amount of the protein of the present invention in the test solution can be determined. The primary reaction and the secondary reaction may be performed in the reverse order, may be performed simultaneously, or may be performed at staggered times. The labeling agent and the method of insolubilization can be in accordance with those described above. In addition, in the immunoassay by the sandwich method, the antibody used for the solid phase antibody or the labeling antibody is not necessarily one kind, and a mixture of two or more kinds of antibodies is used for the purpose of improving measurement sensitivity and the like. You may.
In the method for measuring the protein of the present invention by the sandwich method of the present invention, as the monoclonal antibody of the present invention used in the primary reaction and the secondary reaction, an antibody having a different site to which the protein of the present invention binds is preferably used. That is, the antibody used in the primary reaction and the secondary reaction is preferably, for example, when the antibody used in the secondary reaction recognizes the C-terminal of the protein of the present invention, the antibody used in the primary reaction is preferably An antibody that recognizes, for example, the N-terminal other than the C-terminal is used.
[0048]
The monoclonal antibody of the present invention can be used in a measurement system other than the sandwich method, for example, a competition method, an immunometric method, a nephrometry, or the like.
In the competition method, after the antigen in the test solution and the labeled antigen are allowed to react competitively with the antibody, the unreacted labeled antigen (F) and the labeled antigen (B) bound to the antibody are separated. (B / F separation), the amount of any of B and F is measured, and the amount of antigen in the test solution is quantified. In this reaction method, a soluble antibody is used as the antibody, B / F separation is performed using polyethylene glycol, a liquid phase method using a second antibody against the antibody, or a solid phase antibody is used as the first antibody. A solid-phase method using a soluble antibody as the first antibody and using a solid-phased antibody as the second antibody is used.
In the immunometric method, the antigen in the test solution and the immobilized antigen are subjected to a competitive reaction with a fixed amount of the labeled antibody, and then the solid phase and the liquid phase are separated. And an excess amount of the labeled antibody, and then immobilized antigen is added to bind unreacted labeled antibody to the solid phase, and then the solid phase and the liquid phase are separated. Next, the amount of label in any phase is measured to determine the amount of antigen in the test solution.
In nephelometry, the amount of insoluble sediment produced as a result of an antigen-antibody reaction in a gel or in a solution is measured. Even when the amount of antigen in the test solution is small and only a small amount of sediment is obtained, laser nephrometry utilizing laser scattering is preferably used.
[0049]
In applying these individual immunological measurement methods to the quantification method of the present invention, no special conditions, operations, and the like need to be set. The protein measurement system of the present invention may be constructed by adding ordinary technical considerations of those skilled in the art to ordinary conditions and operation methods in each method. For details of these general technical means, reference can be made to reviews, books, and the like.
For example, Hiroe Irie, "Radio Immunoassay" (Kodansha, published in 1974), Hiroshi Irie, "Radio Immunoassay" (Kodansha, published in 1974), Eiji Ishikawa et al., "Enzyme Immunoassay" (Medical Shoin, Showa Ed. Ishikawa et al., “Enzyme Immunoassay” (2nd edition) (Issue Shoin, 1982), Eiji Ishikawa et al. “Enzyme Immunoassay” (Third Edition), 3rd edition (Medical Shoin, Showa) 62)), "Methods in ENZYMOLOGY" Vol. 70 (Immunochemical Techniques (Part A)), ibid., Vol. 73 (Immunochemical Technologies (Part B)), ibid., Vol. 74 (Immunochemical Technologies (Part C)), ibid., Vol. 84 (Immunochemical Technologies (Part D: Selected Immunoassays)), ibid., Vol. 92 (Immunochemical Technologies) (Part E: Monoclonal Antibodies and General Immunoassay Methods), ibid., Vol. 121 (Immunochemical Technologies (Part I: Hybridoma Technology and Monoclonal Antibodies)) (all published by Academic Press) can be referred to.
As described above, the protein of the present invention can be quantified with high sensitivity by using the antibody of the present invention.
Furthermore, when an increase or decrease in the concentration of the protein of the present invention is detected by quantifying the concentration of the protein of the present invention using the antibody of the present invention, for example, respiratory diseases (eg, chronic obstructive pulmonary disease) (Chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, Hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, Insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with spleen dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis Etc. it is, or it can be diagnosed that it is highly likely to suffer from these disease in the future.
Further, the antibody of the present invention can be used for detecting the protein of the present invention present in a subject such as a body fluid or a tissue. Further, for preparation of an antibody column used for purifying the protein of the present invention, detection of the protein of the present invention in each fraction at the time of purification, analysis of the behavior of the protein of the present invention in test cells, etc. Can be used.
[0050]
(3) Gene diagnostics
The DNA of the present invention can be used, for example, as a probe to produce a human or warm-blooded animal (eg, rat, mouse, guinea pig, rabbit, bird, sheep, pig, cow, horse, cat, dog, monkey, chimpanzee, etc.). Can detect an abnormality (genetic abnormality) in DNA or mRNA encoding the protein of the present invention or a partial peptide thereof in, for example, damage, mutation or decrease in expression of the DNA or mRNA, or decrease in the DNA or mRNA. It is useful as a diagnostic agent for a gene such as increase or overexpression.
The above-described genetic diagnosis using the DNA of the present invention can be performed, for example, by the known Northern hybridization or PCR-SSCP method (Genomics, Vol. 5, pp. 874-879 (1989), Proceedings of the National Academy of Science of the). United States of America, Vol. 86, pp. 2766-2770 (1989)) and the like.
For example, when overexpression or decrease is detected by Northern hybridization or when DNA mutation is detected by PCR-SSCP method, for example, respiratory diseases [eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema ), Diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic) Rhinitis, dry anoritis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc., immune diseases (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, chronic Rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), inflammatory bowel disease, allergic reactions It can be diagnosed that it is highly likely that in such flames.
[0051]
(4) Drug containing antisense polynucleotide
The antisense polynucleotide of the present invention capable of binding complementarily to the DNA of the present invention and suppressing the expression of the DNA has low toxicity, and the function of the protein of the present invention or the function of the DNA of the present invention in vivo (eg, For example, respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cysts) because they can inhibit cell adhesion activity or heparan sulfate proteoglycan binding activity. Dysfibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry prerhinitis, vasomotor rhinitis, gangrene Rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, whole body Erythematosus, atopic dermatitis, leukocyte abnormalities, such as spleen dysfunction or thymus abnormally accompanying immunodeficiency), can be used inflammatory bowel disease, as a prophylactic or therapeutic agent for allergic conjunctivitis. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
When the antisense polynucleotide is used as the prophylactic / therapeutic agent, it can be formulated and administered according to a method known per se.
Also, for example, after inserting the antisense polynucleotide alone or into an appropriate vector such as a retrovirus vector, an adenovirus vector, an adenovirus associated virus vector, and the like, a human or mammal (eg, rat, Rabbits, sheep, pigs, cows, cats, dogs, monkeys, and the like). The antisense polynucleotide can be administered as it is or in the form of a formulation together with a physiologically acceptable carrier such as an auxiliary agent for promoting uptake, and can be administered using a gene gun or a catheter such as a hydrogel catheter. Alternatively, they can be aerosolized and administered locally into the trachea as an inhalant.
Furthermore, for the purpose of improving pharmacokinetics, prolonging the half-life, and improving the efficiency of cellular uptake, the antisense polynucleotide is formulated alone or in combination with a carrier such as liposome (injection), and is used for intravenous, subcutaneous, respiratory, It may be administered to a pulmonary lesion or the like. The dosage of the antisense polynucleotide varies depending on the target disease, the administration subject, the administration route, and the like. For example, when the antisense polynucleotide of the present invention is administered for the purpose of treating emphysema, generally, the adult ( (Body weight 60 kg), about 0.1 to 100 mg of the antisense polynucleotide is administered per day.
Similarly to the above-mentioned antisense polynucleotide, a double-stranded RNA containing a part of the RNA encoding the protein of the present invention, a ribozyme containing a part of the RNA encoding the protein of the present invention, and the like also include the gene of the present invention. Can be suppressed, and the function of the protein used in the present invention or the DNA used in the present invention in a living body can be suppressed, for example, respiratory diseases [eg, chronic obstructive pulmonary disease (chronic Bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic) Rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, sclerosis) Len syndrome, insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis, etc. It can be used as an agent. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
The double-stranded RNA can be produced by designing based on the sequence of the polynucleotide of the present invention according to a known method (eg, Nature, 411, 494, 2001).
A ribozyme can be designed and produced based on the sequence of the polynucleotide of the present invention according to a known method (eg, TRENDS in Molecular Medicine, Vol. 7, pp. 221, 2001). For example, it can be produced by linking a known ribozyme to a part of RNA encoding the protein of the present invention. As a part of the RNA encoding the protein of the present invention, a portion (RNA fragment) close to a cleavage site on the RNA of the present invention, which can be cleaved by a known ribozyme, can be mentioned.
When the above-mentioned double-stranded RNA or ribozyme is used as the above-mentioned prophylactic / therapeutic agent, it can be formulated and administered in the same manner as an antisense polynucleotide.
[0052]
(5) Drug containing the antibody of the present invention
Antibodies of the present invention having an activity of neutralizing the activity of the protein of the present invention include, for example, respiratory diseases [eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cysts Dysfibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry prerhinitis, vasomotor rhinitis, gangrene Rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocytes Abnormalities, spleen insufficiency or immunodeficiency associated with thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis and the like. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
The antibodies of the present invention can be administered as such or as a suitable pharmaceutical composition. The pharmaceutical composition used for the administration contains the antibody or a salt thereof and a pharmacologically acceptable carrier, diluent or excipient. Such compositions are provided in dosage forms suitable for oral or parenteral administration.
That is, for example, compositions for oral administration include solid or liquid dosage forms, specifically tablets (including sugar-coated tablets and film-coated tablets), pills, granules, powders, capsules (soft capsules and the like). Syrup, emulsion, suspension and the like. Such a composition is produced by a known method and contains a carrier, diluent or excipient commonly used in the field of pharmaceuticals. For example, lactose, starch, sucrose, magnesium stearate and the like are used as carriers and excipients for tablets.
As the composition for parenteral administration, for example, injections, suppositories, etc. are used, and the injections are in the form of intravenous injections, subcutaneous injections, intradermal injections, intramuscular injections, intravenous injections and the like. Is included. Such injections are prepared according to a known method, for example, by dissolving, suspending or emulsifying the antibody or a salt thereof in a sterile aqueous or oily liquid commonly used for injections. As an aqueous liquid for injection, for example, physiological saline, isotonic solution containing glucose and other auxiliary agents and the like are used, and suitable solubilizing agents, for example, alcohol (eg, ethanol), polyalcohol (eg, Propylene glycol, polyethylene glycol), nonionic surfactants (eg, polysorbate 80, HCO-50 (polyoxyethylene (50 mol) add-on of hydro- genated castor oil)) and the like may be used in combination. As the oily liquid, for example, sesame oil, soybean oil, and the like are used, and benzyl benzoate, benzyl alcohol, and the like may be used in combination as a solubilizing agent. The prepared injection is usually filled in an appropriate ampoule. Suppositories to be used for rectal administration are prepared by mixing the above antibody or a salt thereof with a conventional suppository base.
The above-mentioned oral or parenteral pharmaceutical composition is conveniently prepared in a unit dosage form so as to be compatible with the dosage of the active ingredient. Examples of such dosage unit dosage forms include tablets, pills, capsules, injections (ampoules), suppositories, and the like. Usually, each dosage unit dosage form has a dosage of 5 to 500 mg, especially 5 to 100 mg for an injection. Other dosage forms preferably contain 10 to 250 mg of the above antibody.
Each of the above-mentioned compositions may contain another active ingredient as long as the composition does not cause an undesirable interaction with the antibody.
The prophylactic / therapeutic agent for the above-mentioned diseases containing the antibody of the present invention has low toxicity and is used as it is as a liquid or as a pharmaceutical composition of an appropriate dosage form, in humans or mammals (eg, rat, rabbit, sheep, pig, It can be administered orally or parenterally (eg, intravenously) to cattle, cats, dogs, monkeys, and the like. The dose varies depending on the administration subject, target disease, symptoms, administration route, and the like. For example, when used for the treatment or prevention of emphysema in adults, the antibody of the present invention is usually administered in a dose of 0 to 1 dose. 0.01 to 20 mg / kg body weight, preferably about 0.1 to 10 mg / kg body weight, more preferably about 0.1 to 5 mg / kg body weight, about 1 to 5 times a day, preferably 1 to 3 times a day. It is convenient to administer as an injection about once. In the case of other parenteral administration and oral administration, an equivalent amount can be administered. If the symptoms are particularly severe, the dose may be increased according to the symptoms.
The antibody of the present invention can be used, for example, for respiratory diseases [eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, lung fibrosis Disease), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry pronasitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immunology Diseases (eg, associated with myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistance diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, splenic dysfunction or thymic abnormalities It is also useful as a diagnostic for inflammatory bowel disease, allergic conjunctivitis, etc.
[0053]
(6) The “prophylactic / therapeutic agent for respiratory diseases comprising a compound having an activity of regulating heparan sulfate proteoglycan binding activity or a salt thereof” of the present invention
The “compound having an activity of regulating heparan sulfate proteoglycan binding activity” may be any compound having an activity of regulating heparan sulfate proteoglycan binding activity, such as a respiratory disease (eg, chronic obstructive pulmonary disease ( Chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, thickening) Rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc., immune diseases (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin) Resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), Diseases bowel disease, can be used as a prophylactic or therapeutic agent for allergic conjunctivitis. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
The prophylactic / therapeutic agent is produced in the same manner as described above.
[0054]
(7) DNA transfer animal
The present invention relates to a non-protein having a DNA encoding an exogenous protein of the present invention (hereinafter abbreviated as the exogenous DNA of the present invention) or a mutant DNA thereof (sometimes abbreviated as the exogenous mutant DNA of the present invention). A human mammal is provided.
That is, the present invention
(1) a non-human mammal having the exogenous DNA of the present invention or a mutant DNA thereof,
(2) the animal according to (1), wherein the non-human mammal is a rodent;
(3) The animal according to (2), wherein the rodent is a mouse or a rat, and
(4) It is intended to provide a recombinant vector containing the exogenous DNA of the present invention or its mutant DNA and capable of being expressed in mammals.
Non-human mammals having the exogenous DNA of the present invention or the mutant DNA thereof (hereinafter abbreviated as the DNA-transferred animal of the present invention) can be used for non-fertilized eggs, fertilized eggs, germ cells including spermatozoa and their progenitor cells, And preferably at the stage of embryonic development in non-human mammal development (more preferably at the stage of single cells or fertilized eggs and generally before the 8-cell stage), the calcium phosphate method, the electric pulse method, the lipofection method, the agglutination method, It can be produced by transferring a target DNA by a microinjection method, a particle gun method, a DEAE-dextran method, or the like. Further, by the DNA transfer method, the exogenous DNA of the present invention can be transferred to somatic cells, organs of living organisms, tissue cells, and the like, and can be used for cell culture, tissue culture, and the like. The DNA-transferred animal of the present invention can also be produced by fusing the above-mentioned germ cells with a cell fusion method known per se.
As the non-human mammal, for example, cow, pig, sheep, goat, rabbit, dog, cat, guinea pig, hamster, mouse, rat and the like are used. Among them, rodents, which are relatively short in ontogeny and biological cycle in terms of preparation of disease animal model systems, and are easy to breed, especially mice (for example, hybrids such as C57BL / 6 strain and DBA2 strain as pure strains) B6C3F as a system ₁ System, BDF ₁ System, B6D2F ₁ Strain, BALB / c strain, ICR strain, etc.) or rat (eg, Wistar, SD etc.) is preferred.
"Mammals" in a recombinant vector that can be expressed in mammals include humans in addition to the above-mentioned non-human mammals.
[0055]
The exogenous DNA of the present invention refers to the DNA of the present invention once isolated and extracted from a mammal, not the DNA of the present invention originally possessed by a non-human mammal.
As the mutant DNA of the present invention, those having a mutation (for example, mutation) in the base sequence of the original DNA of the present invention, specifically, base addition, deletion, substitution with another base, etc. The resulting DNA or the like is used, and also includes abnormal DNA.
The abnormal DNA means a DNA that expresses an abnormal protein of the present invention, and for example, a DNA that expresses a protein that suppresses the function of the normal protein of the present invention is used.
The exogenous DNA of the present invention may be derived from a mammal that is the same or different from the animal of interest. In transferring the DNA of the present invention to a target animal, it is generally advantageous to use the DNA as a DNA construct linked downstream of a promoter capable of being expressed in animal cells. For example, when the human DNA of the present invention is transferred, DNA derived from various mammals (eg, rabbits, dogs, cats, guinea pigs, hamsters, rats, mice, etc.) having the DNA of the present invention having high homology thereto is expressed. Highly expressing the DNA of the present invention by microinjecting a DNA construct (eg, vector, etc.) in which the human DNA of the present invention is bound downstream of various promoters that can be made into a fertilized egg of a target mammal, for example, a mouse fertilized egg. DNA-transferring mammals can be created.
[0056]
Examples of the expression vector of the protein of the present invention include plasmids derived from Escherichia coli, plasmids derived from Bacillus subtilis, plasmids derived from yeast, bacteriophages such as λ phage, retroviruses such as Moloney leukemia virus, animal viruses such as vaccinia virus or baculovirus. Are used. Among them, a plasmid derived from Escherichia coli, a plasmid derived from Bacillus subtilis or a plasmid derived from yeast is preferably used.
Examples of the promoter that regulates the DNA expression include, but are not limited to, (1) a promoter of a DNA derived from a virus (eg, simian virus, cytomegalovirus, Moloney leukemia virus, JC virus, breast cancer virus, polio virus, etc.); ▼ Promoters derived from various mammals (human, rabbit, dog, cat, guinea pig, hamster, rat, mouse, etc.), for example, albumin, insulin II, uroplakin II, elastase, erythropoietin, endothelin, muscle creatine kinase, glial fibrillary acid Protein, glutathione S-transferase, platelet-derived growth factor β, keratins K1, K10 and K14, collagen type I and type II, cyclic AMP-dependent protein kinase βI subunit, dyst Lophine, tartrate-resistant alkaline phosphatase, atrial natriuretic factor, endothelial receptor tyrosine kinase (commonly abbreviated as Tie2), sodium potassium adenosine 3 kinase (Na, K-ATPase), neurofilament light chain, metallothionein I and IIA, metalloproteinase 1 tissue inhibitor, MHC class I antigen (H-2L), H-ras, renin, dopamine β-hydroxylase, thyroid peroxidase (TPO), peptide chain elongation factor 1α (EF-1α), β actin , Α and β myosin heavy chain, myosin light chain 1 and 2, myelin basic protein, thyroglobulin, Thy-1, immunoglobulin, heavy chain variable region (VNP), serum amyloid P component, myoglobin, troponin C, smooth muscle α Kuching, pre-pro-enkephalin A, such as a promoter, such as vasopressin is used. Among them, a cytomegalovirus promoter capable of high expression throughout the body, a human peptide chain elongation factor 1α (EF-1α) promoter, a human and chicken β-actin promoter, and the like are preferable.
The vector preferably has a sequence that terminates transcription of the target messenger RNA in a DNA-transferred mammal (generally called a terminator). For example, a sequence of each DNA derived from a virus and various mammals can be used. A simian virus SV40 terminator or the like is preferably used.
[0057]
In addition, a splicing signal of each DNA, an enhancer region, a part of an intron of a eukaryotic DNA, and the like are placed 5 ′ upstream of the promoter region, between the promoter region and the translation region, or between the translation region for the purpose of further expressing the desired foreign DNA. It is also possible to connect 3 ′ downstream of the above depending on the purpose.
The normal translation region of the protein of the present invention can be obtained from liver, kidney, thyroid cells, fibroblast-derived DNA derived from humans or various mammals (eg, rabbits, dogs, cats, guinea pigs, hamsters, rats, mice, etc.) and commercially available DNAs. From a variety of genomic DNA libraries, or as a starting material, a complementary DNA prepared by known methods from RNA derived from liver, kidney, thyroid cells, and fibroblasts. In addition, a translation region obtained by mutating a translation region of a normal protein obtained from the above-described cells or tissues by a point mutagenesis method can be used for the exogenous abnormal DNA.
The translation region can be prepared as a DNA construct that can be expressed in a transposed animal by a conventional DNA engineering technique in which it is ligated downstream of the above-mentioned promoter and, if desired, upstream of the transcription termination site.
Transfer of the exogenous DNA of the present invention at the fertilized egg cell stage is ensured to be present in all germ cells and somatic cells of the target mammal. The presence of the exogenous DNA of the present invention in the germinal cells of the produced animal after DNA transfer means that all the progeny of the produced animal retain the exogenous DNA of the present invention in all of the germinal cells and somatic cells. means. The offspring of such animals that have inherited the exogenous DNA of the present invention have the exogenous DNA of the present invention in all of their germ cells and somatic cells.
The non-human mammal to which the exogenous normal DNA of the present invention has been transferred can be subcultured in a normal breeding environment as an animal having the DNA after confirming that the exogenous DNA is stably retained by mating. .
Transfer of the exogenous DNA of the present invention at the fertilized egg cell stage is ensured to be present in excess in all germ cells and somatic cells of the target mammal. Excessive presence of the exogenous DNA of the present invention in germ cells of a produced animal after DNA transfer means that all offspring of the produced animal have an excessive amount of the exogenous DNA of the present invention in all of their germ cells and somatic cells. Means Progeny of such animals that have inherited the exogenous DNA of the present invention have an excess of the exogenous DNA of the present invention in all of their germinal and somatic cells.
By obtaining a homozygous animal having the introduced DNA on both homologous chromosomes and mating the male and female animals, all offspring can be bred to have the DNA in excess.
[0058]
The non-human mammal having the normal DNA of the present invention expresses the normal DNA of the present invention at a high level and promotes the function of the endogenous normal DNA to eventually cause hyperactivity of the protein of the present invention. Occasionally, it can be used as a disease model animal. For example, using the normal DNA-transferred animal of the present invention, it is possible to elucidate the pathological mechanism of hyperactivity of the protein of the present invention and diseases associated with the protein of the present invention, and to examine a method for treating these diseases. It is possible.
Further, since the mammal into which the exogenous normal DNA of the present invention has been transferred has an increased symptom of the free protein of the present invention, a preventive / therapeutic agent for a disease associated with the protein of the present invention, for example, a respiratory disease [ Eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever) , Acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, glomerulonephritis, multiple Sclerosis, Sjogren's syndrome, insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), inflammatory Disease, can also be utilized in the screening test prophylactic or therapeutic agent such as allergic conjunctivitis.
On the other hand, a non-human mammal having the exogenous abnormal DNA of the present invention can be subcultured in an ordinary breeding environment as an animal having the DNA after confirming that the exogenous DNA is stably maintained by mating. Furthermore, the desired foreign DNA can be used as a raw material by incorporating it into the aforementioned plasmid. The DNA construct with the promoter can be prepared by a usual DNA engineering technique. The transfer of the abnormal DNA of the present invention at the fertilized egg cell stage is ensured to be present in all germ cells and somatic cells of the target mammal. The presence of the abnormal DNA of the present invention in the germinal cells of the produced animal after DNA transfer means that all the offspring of the produced animal have the abnormal DNA of the present invention in all of its germ cells and somatic cells. The progeny of such animals that have inherited the exogenous DNA of the present invention have the abnormal DNA of the present invention in all of their germinal and somatic cells. A homozygous animal having the introduced DNA on both homologous chromosomes is obtained, and by crossing these male and female animals, it is possible to breed the cells so that all offspring have the DNA.
[0059]
The non-human mammal having the abnormal DNA of the present invention, in which the abnormal DNA of the present invention is highly expressed, inhibits the function of endogenous normal DNA, and finally, the functionally inactive form of the protein of the present invention. It can be refractory and can be used as a model animal for the disease. For example, using the abnormal DNA-transferred animal of the present invention, it is possible to elucidate the pathological mechanism of the function-inactive refractory of the protein of the present invention and to examine a method for treating this disease.
Further, as a specific possibility, the abnormal DNA-highly expressing animal of the present invention exhibits a function of inhibiting the normal protein function (dominant negative action) by the abnormal protein of the present invention in the inactive refractory disease of the protein of the present invention. A model to elucidate. In addition, since the mammal to which the foreign abnormal DNA of the present invention has been transferred has an increased symptom of the free protein of the present invention, a prophylactic / therapeutic agent for the protein of the present invention or a functionally inactive refractory disease, for example, Disease (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, Hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, glomerulonephritis) , Multiple sclerosis, Sjogren's syndrome, insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities) Inflammatory bowel disease, in screening test for preventive and therapeutic agent for allergic conjunctivitis are available.
In addition, other possible uses of the above two DNA-transferred animals of the present invention include, for example,
(1) Use as a cell source for tissue culture,
(2) A peptide specifically expressed or activated by the protein of the present invention by directly analyzing DNA or RNA in the tissue of the DNA-transferred animal of the present invention or analyzing a peptide tissue expressed by the DNA Analysis of the relationship with
{Circle around (3)} The cells of a tissue having DNA are cultured by standard tissue culture techniques, and these are used to study the function of cells from tissues that are generally difficult to culture.
(4) screening for a drug that enhances the function of the cell by using the cell described in (3) above, and
{Circle around (5)} Isolation and purification of the mutant protein of the present invention and production of its antibody can be considered.
[0060]
Furthermore, using the DNA-transferred animal of the present invention, it is possible to examine clinical symptoms of a disease associated with the protein of the present invention, including a functionally inactive refractory disease of the protein of the present invention, and the like. More detailed pathological findings in each organ of the disease model related to the disease can be obtained, which can contribute to the development of a new treatment method, and further to the research and treatment of a secondary disease caused by the disease.
In addition, it is possible to take out each organ from the DNA-transferred animal of the present invention, cut it into small pieces, and then use a proteolytic enzyme such as trypsin to obtain the released DNA-transferred cells, culture them, or systematize the cultured cells. . Furthermore, it is possible to examine the specificity of the protein-producing cell of the present invention, its relationship with apoptosis, differentiation or proliferation, or its signal transduction mechanism, and its abnormalities. It is an effective research material for
Further, in order to develop a therapeutic agent for a disease associated with the protein of the present invention, including a functionally inactive refractory disease of the protein of the present invention, using the DNA-transferred animal of the present invention, It is possible to provide an effective and rapid screening method for a therapeutic agent for the disease by using a method or the like. In addition, using the transgenic animal of the present invention or the exogenous DNA expression vector of the present invention, it is possible to examine and develop a DNA treatment method for diseases associated with the protein of the present invention.
[0061]
(8) Knockout animal
The present invention provides a non-human mammalian embryonic stem cell in which the DNA of the present invention has been inactivated, and a non-human mammal deficient in expression of the DNA of the present invention.
That is, the present invention
(1) a non-human mammalian embryonic stem cell in which the DNA of the present invention has been inactivated,
(2) The embryonic stem cell according to (1), wherein the DNA is inactivated by introducing a reporter gene (eg, a β-galactosidase gene derived from E. coli).
(3) the embryonic stem cell according to (1), which is neomycin-resistant;
(4) the embryonic stem cell according to (1), wherein the non-human mammal is a rodent;
(5) The embryonic stem cell according to (4), wherein the rodent is a mouse,
(6) a non-human mammal deficient in expression of the DNA of the present invention, wherein the DNA is inactivated;
(7) The DNA is inactivated by introducing a reporter gene (eg, a β-galactosidase gene derived from Escherichia coli), and the reporter gene can be expressed under the control of a promoter for the DNA of the present invention (6). The non-human mammal according to the item,
(8) the non-human mammal according to (6), wherein the non-human mammal is a rodent;
(9) The non-human mammal according to (8), wherein the rodent is a mouse, and
(10) A method for screening a compound or a salt thereof that promotes or inhibits promoter activity on DNA of the present invention, which comprises administering a test compound to the animal according to (7) and detecting expression of a reporter gene. I will provide a.
[0062]
A non-human mammalian embryonic stem cell in which the DNA of the present invention has been inactivated is a DNA which is artificially mutated to the DNA of the present invention possessed by the non-human mammal, thereby suppressing the expression ability of the DNA, or By substantially losing the activity of the protein of the present invention encoded by the DNA, the DNA does not substantially have the ability to express the protein of the present invention (hereinafter, may be referred to as the knockout DNA of the present invention). ) Non-human mammalian embryonic stem cells (hereinafter abbreviated as ES cells).
As the non-human mammal, the same one as described above is used.
The method of artificially mutating the DNA of the present invention can be performed, for example, by deleting a part or all of the DNA sequence and inserting or substituting another DNA by a genetic engineering technique. With these mutations, the knockout DNA of the present invention may be prepared, for example, by shifting the codon reading frame or disrupting the function of the promoter or exon.
[0063]
Specific examples of the non-human mammalian embryonic stem cells in which the DNA of the present invention has been inactivated (hereinafter abbreviated as the DNA-inactivated ES cells of the present invention or the knockout ES cells of the present invention) include, for example, The DNA of the present invention possessed by a non-human mammal is isolated and its exon portion is a drug resistance gene typified by a neomycin resistance gene or a hygromycin resistance gene, or lacZ (β-galactosidase gene), cat (chloramphenicol acetyl). A reporter gene or the like typified by a transferase gene) to disrupt the exon function, or insert a DNA sequence that terminates gene transcription into an intron between exons (for example, a polyA addition signal); Inability to synthesize complete messenger RNA Thus, a DNA strand having a DNA sequence constructed so as to eventually destroy the gene (hereinafter abbreviated as a targeting vector) is introduced into the chromosome of the animal by, for example, homologous recombination, and the resulting ES cells PCR using the DNA sequence on or near the DNA of the present invention as a probe, and using the DNA sequence on the targeting vector and the DNA sequence in the neighboring region other than the DNA of the present invention used for the preparation of the targeting vector as primers And selecting the knockout ES cells of the present invention.
As the ES cells from which the DNA of the present invention is inactivated by the homologous recombination method or the like, for example, those already established as described above may be used, or according to the known Evans and Kaufma method. It may be a newly established one. For example, in the case of mouse ES cells, currently, 129-line ES cells are generally used. For example, for the purpose of obtaining ES cells in which BDF is clearly known, for example, BDF in which the number of eggs collected by C57BL / 6 mice or C57BL / 6 has been improved by hybridization with DBA / 2 ₁ Mouse (F of C57BL / 6 and DBA / 2) ₁ ) Can also be used favorably. BDF ₁ In addition to the advantage that the number of eggs collected and the eggs are robust, the mice have C57BL / 6 mice as a background, and thus, the ES cells obtained using the C57BL / 6 mice were used to produce C57BL / 6 mice. / 6 mice can be advantageously used in that the genetic background can be replaced by C57BL / 6 mice by backcrossing.
In addition, when ES cells are established, blastocysts 3.5 days after fertilization are generally used. In addition, a large number of blastocysts can be efficiently obtained by collecting embryos at the 8-cell stage and culturing them until blastocysts are used. Early embryos can be obtained.
Either male or female ES cells may be used, but generally male ES cells are more convenient for producing a germline chimera. It is also desirable to discriminate between males and females as soon as possible in order to reduce cumbersome culture labor.
[0064]
As a method for determining the sex of ES cells, for example, a method of amplifying and detecting a gene in a sex-determining region on the Y chromosome by a PCR method can be mentioned. If this method is used, it is conventionally necessary to perform about 10 karyotype analyses. ⁶ Since the number of ES cells is required, the number of ES cells of about 1 colony (approximately 50) is sufficient, so that primary selection of ES cells in the early stage of culture can be performed by discriminating between male and female. In addition, by enabling selection of male cells at an early stage, labor in the initial stage of culture can be significantly reduced.
The secondary selection can be performed, for example, by confirming the number of chromosomes by the G-banding method. The number of chromosomes in the obtained ES cells is desirably 100% of the normal number. However, when it is difficult due to physical operations at the time of establishment, after knocking out the gene of the ES cells, the normal cells (for example, chromosomes in mice) are knocked out. It is desirable to clone again into cells (number 2n = 40).
The embryonic stem cell line obtained in this way usually has very good growth properties, but it must be carefully subcultured because it tends to lose its ontogenic ability. For example, on a suitable feeder cell such as STO fibroblast in the presence of LIF (1 to 10,000 U / ml) in a carbon dioxide incubator (preferably 5% carbon dioxide, 95% air or 5% oxygen, 5% The cells are cultured by a method such as culturing at about 37 ° C. in carbon dioxide gas and 90% air. At the time of subculture, for example, trypsin / EDTA solution (usually 0.001 to 0.5% trypsin / 0.1 to 5 mM EDTA, Preferably, a method is used in which cells are made into single cells by treatment with about 0.1% trypsin / 1 mM EDTA and seeded on freshly prepared feeder cells. Such passage is usually carried out every 1 to 3 days. At this time, it is desirable to observe the cells and, if any morphologically abnormal cells are found, discard the cultured cells.
ES cells are differentiated into various types of cells, such as parietal muscle, visceral muscle, and cardiac muscle, by monolayer culture up to high density or suspension culture until cell clumps are formed under appropriate conditions. [M. J. Evans and M.E. H. Kaufman, Nature 292, 154, 1981; R. Martin Proc. Natl. Acad. Sci. U. S. A. 78, 7634, 1981; C. Doetschman et al., Journal of Embryology and Experimental Morphology, Vol. 87, p. 27, 1985], that the DNA-deficient cell of the present invention obtained by differentiating the ES cell of the present invention is characterized by in vitro Is useful in cell biological studies of the protein of the present invention.
[0065]
The non-human mammal deficient in DNA expression of the present invention can be distinguished from a normal animal by measuring the mRNA level of the animal using a known method and indirectly comparing the expression level.
As the non-human mammal, those similar to the aforementioned can be used.
The non-human mammal deficient in expression of the DNA of the present invention is, for example, a DNA in which the targeting vector prepared as described above is introduced into mouse embryonic stem cells or mouse egg cells, and the DNA of the targeting vector is inactivated by the introduction. The DNA of the present invention can be knocked out by homologous recombination in which the sequence replaces the DNA of the present invention on the chromosome of mouse embryonic stem cells or mouse egg cells by homologous recombination.
Cells in which the DNA of the present invention has been knocked out can be used as a DNA sequence on a Southern hybridization analysis or targeting vector using the DNA sequence on or near the DNA of the present invention as a probe, and the DNA of the present invention derived from the mouse used for the targeting vector. It can be determined by analysis by PCR using a DNA sequence of a nearby region other than DNA as a primer. When non-human mammalian embryonic stem cells are used, a cell line in which the DNA of the present invention has been inactivated by gene homologous recombination is cloned, and the cells are cultured at an appropriate time, for example, at the 8-cell stage of non-human mammalian cells. The chimeric embryo is injected into an animal embryo or blastocyst, and the resulting chimeric embryo is transplanted into the uterus of the pseudopregnant non-human mammal. The produced animal is a chimeric animal comprising both cells having the normal DNA locus of the present invention and cells having the artificially mutated DNA locus of the present invention. When a part of the germ cells of the chimeric animal has a mutated DNA locus of the present invention, all tissues are artificially mutated from a population obtained by crossing such a chimeric individual with a normal individual. It can be obtained by selecting individuals composed of cells having the added DNA locus of the present invention, for example, by judging coat color or the like. The individual thus obtained is usually an individual with a heterozygous expression of the protein of the present invention, which is crossed with an individual with a heterozygous expression of the protein of the present invention, and homozygous expression of the protein of the present invention from their offspring. Defective individuals can be obtained.
[0066]
In the case of using an egg cell, for example, a transgenic non-human mammal having a targeting vector introduced into a chromosome can be obtained by injecting a DNA solution into a nucleus of an egg by a microinjection method, and these transgenic non-human mammals can be obtained. Compared to mammals, they can be obtained by selecting those having a mutation in the DNA locus of the present invention by homologous recombination.
In this manner, the individual in which the DNA of the present invention is knocked out can be bred in an ordinary breeding environment after confirming that the DNA of the animal obtained by the breeding is also knocked out.
Further, the acquisition and maintenance of the germ line may be performed according to a conventional method. That is, by crossing male and female animals having the inactivated DNA, a homozygous animal having the inactivated DNA on both homologous chromosomes can be obtained. The obtained homozygous animal can be efficiently obtained by rearing the mother animal in such a manner that there are one normal animal and one homozygote. By mating male and female heterozygous animals, homozygous and heterozygous animals having the inactivated DNA are bred and subcultured.
The non-human mammalian embryonic stem cells in which the DNA of the present invention has been inactivated are extremely useful for producing a non-human mammal deficient in expressing the DNA of the present invention.
In addition, since the non-human mammal deficient in expression of the DNA of the present invention lacks various biological activities that can be induced by the protein of the present invention, a model of a disease caused by inactivation of the biological activity of the protein of the present invention. Therefore, it is useful for investigating the causes of these diseases and examining treatment methods.
[0067]
(8a) A method for screening a compound having a therapeutic / preventive effect on diseases caused by DNA deficiency or damage of the present invention
The non-human mammal deficient in expression of the DNA of the present invention can be used for screening for a compound having a therapeutic / preventive effect against diseases caused by deficiency or damage of the DNA of the present invention.
That is, the present invention is characterized by administering a test compound to a non-human mammal deficient in expressing the DNA of the present invention, and observing and measuring a change in the animal. Diseases, for example, respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, , Allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc., immune diseases (eg, myasthenia gravis) Disease, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistance diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities) Inflammatory bowel disease, provides a method of screening a compound or its salt having a therapeutic or prophylactic effect for such allergic conjunctivitis.
Examples of the non-human mammal deficient in expressing DNA of the present invention used in the screening method include the same as described above.
Test compounds include, for example, peptides, proteins, non-peptidic compounds, synthetic compounds, fermentation products, cell extracts, plant extracts, animal tissue extracts, plasma, and the like. These compounds are novel compounds. Or a known compound.
Specifically, a non-human mammal deficient in expression of the DNA of the present invention is treated with a test compound, compared with an untreated control animal, and tested using changes in each organ, tissue, disease symptoms, etc. of the animal as an index. The therapeutic / preventive effects of the compounds can be tested.
As a method of treating a test animal with a test compound, for example, oral administration, intravenous injection and the like are used, and it can be appropriately selected according to the symptoms of the test animal, the properties of the test compound, and the like. The dose of the test compound can be appropriately selected according to the administration method, the properties of the test compound, and the like.
[0068]
For example, respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergy) Rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune diseases (eg, myasthenia gravis, Glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistance diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with splenic dysfunction or thymic abnormalities), inflammatory bowel disease When screening for a compound having a therapeutic / preventive effect against allergic conjunctivitis or the like, a test compound is administered to a non-human mammal deficient in expressing the DNA of the present invention. The difference of emphysema of the given group and the lung, such as differences in respiratory function over time observed in the tissue.
In the screening method, when the test compound is administered to a test animal, if the disease symptom of the test animal is improved by about 10% or more, preferably about 30% or more, more preferably about 50% or more, the test compound is administered. It can be selected as a compound having a therapeutic / preventive effect on the above diseases.
The compound obtained by using the screening method is a compound selected from the test compounds described above, and has a therapeutic / preventive effect on a disease caused by deficiency or damage of the protein of the present invention. It can be used as a drug for safe and low toxic prophylactic / therapeutic agents. Furthermore, compounds derived from the compounds obtained by the above screening can be used in the same manner.
The compound obtained by the screening method may form a salt. Examples of the salt of the compound include physiologically acceptable acids (eg, inorganic acids, organic acids, etc.) and bases (eg, alkali metals, etc.). ) Is used, and a physiologically acceptable acid addition salt is particularly preferable. Such salts include, for example, salts with inorganic acids (eg, hydrochloric acid, phosphoric acid, hydrobromic acid, sulfuric acid, etc.) or organic acids (eg, acetic acid, formic acid, propionic acid, fumaric acid, maleic acid, For example, salts with succinic acid, tartaric acid, citric acid, malic acid, oxalic acid, benzoic acid, methanesulfonic acid, benzenesulfonic acid, and the like are used.
A drug containing the compound or a salt thereof obtained by the screening method can be produced in the same manner as the above-mentioned drug containing the protein of the present invention.
Since the preparation thus obtained is safe and low toxic, it can be used, for example, in humans or mammals (eg, rat, mouse, guinea pig, rabbit, sheep, pig, cow, horse, cat, dog, monkey, etc.). Can be administered.
The dose of the compound or a salt thereof varies depending on the target disease, the administration subject, the administration route, and the like. For example, when the compound is orally administered, in general, in an adult (with a body weight of 60 kg) emphysema patient, About 0.1-100 mg, preferably about 1.0-50 mg, more preferably about 1.0-20 mg of the compound is administered per day. When administered parenterally, the single dose of the compound varies depending on the administration subject, target disease, and the like. For example, the compound is usually administered as an injection to an adult (with a body weight of 60 kg) emphysema patient. If so, it is convenient to administer about 0.01 to 30 mg, preferably about 0.1 to 20 mg, more preferably about 0.1 to 10 of the compound per day by intravenous injection. In the case of other animals, the amount can be administered in terms of the weight per 60 kg.
[0069]
(8b) Method for screening for a compound that promotes or inhibits the activity of a promoter for the DNA of the present invention
The present invention provides a compound which promotes or inhibits the activity of a promoter for the DNA of the present invention, which comprises administering a test compound to a non-human mammal deficient in expressing the DNA of the present invention, and detecting the expression of a reporter gene, or a compound thereof. A method for screening a salt is provided.
In the above-mentioned screening method, the non-human mammal deficient in expression of DNA of the present invention may be a non-human mammal deficient in expression of DNA of the present invention in which the DNA of the present invention is inactivated by introducing a reporter gene, A reporter gene that can be expressed under the control of a promoter for the DNA of the present invention is used.
Examples of the test compound include the same compounds as described above.
As the reporter gene, the same one as described above is used, and a β-galactosidase gene (lacZ), a soluble alkaline phosphatase gene, a luciferase gene and the like are preferable.
In a non-human mammal deficient in expression of the DNA of the present invention in which the DNA of the present invention is replaced with a reporter gene, since the reporter gene is under the control of the promoter for the DNA of the present invention, the expression of the substance encoded by the reporter gene is traced. By doing so, the activity of the promoter can be detected.
For example, when a part of the DNA region encoding the protein of the present invention is replaced with a β-galactosidase gene (lacZ) derived from Escherichia coli, the tissue that expresses the protein of the present invention originally replaces the protein of the present invention. Β-galactosidase is expressed. Therefore, for example, the present invention can be easily performed by staining with a reagent serving as a substrate for β-galactosidase such as 5-bromo-4-chloro-3-indolyl-β-galactopyranoside (X-gal). Can be observed in the animal body. Specifically, the protein-deficient mouse of the present invention or a tissue section thereof is fixed with glutaraldehyde or the like, washed with phosphate buffered saline (PBS), and then stained with X-gal at room temperature or around 37 ° C. After reacting for about 30 minutes to 1 hour, the β-galactosidase reaction may be stopped by washing the tissue specimen with a 1 mM EDTA / PBS solution, and coloration may be observed. Further, mRNA encoding lacZ may be detected according to a conventional method.
The compound or a salt thereof obtained by using the above-mentioned screening method is a compound selected from the above-mentioned test compounds, and is a compound that promotes or inhibits the promoter activity for the DNA of the present invention.
The compound obtained by the screening method may form a salt, and the salt of the compound may include a physiologically acceptable acid (eg, an inorganic acid) and a base (eg, an alkali metal). Are used, and especially preferred are physiologically acceptable acid addition salts. Such salts include, for example, salts with inorganic acids (eg, hydrochloric acid, phosphoric acid, hydrobromic acid, sulfuric acid, etc.) or organic acids (eg, acetic acid, formic acid, propionic acid, fumaric acid, maleic acid, For example, salts with succinic acid, tartaric acid, citric acid, malic acid, oxalic acid, benzoic acid, methanesulfonic acid, benzenesulfonic acid, and the like are used.
[0070]
The compound or its salt that promotes or inhibits the promoter activity of the DNA of the present invention or the salt thereof can regulate the expression of the protein of the present invention and regulate the function of the protein. Diseases (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis) , Hypertrophic rhinitis, atrophic rhinitis, dry rhinitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome) , Insulin-resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with spleen dysfunction or thymic abnormalities), inflammatory bowel disease It can be used as a prophylactic or therapeutic agent for allergic conjunctivitis. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
Furthermore, compounds derived from the compounds obtained by the above screening can be used in the same manner.
A drug containing the compound or a salt thereof obtained by the screening method can be produced in the same manner as the above-mentioned drug containing the protein of the present invention or a salt thereof.
Since the preparation thus obtained is safe and low toxic, it can be used, for example, in humans or mammals (eg, rat, mouse, guinea pig, rabbit, sheep, pig, cow, horse, cat, dog, monkey, etc.). Can be administered.
The dose of the compound or a salt thereof varies depending on the target disease, the subject to be administered, the administration route, and the like. For example, when the compound of the present invention that inhibits the promoter activity for DNA is orally administered, generally, the adult (body weight) In a patient with emphysema (as 60 kg), about 0.1-100 mg, preferably about 1.0-50 mg, more preferably about 1.0-20 mg of the compound is administered per day. When administered parenterally, the single dose of the compound varies depending on the administration subject, target disease, and the like. For example, the compound of the present invention that inhibits the promoter activity for DNA is usually administered in the form of an injection to an adult ( When administered to a patient with emphysema (as 60 kg), about 0.01 to 30 mg, preferably about 0.1 to 20 mg, more preferably about 0.1 to 10 mg of the compound is administered intravenously per day. It is convenient to do so. In the case of other animals, the amount can be administered in terms of 60 kg.
As described above, the non-human mammal deficient in expression of the DNA of the present invention is extremely useful for screening for a compound or a salt thereof that promotes or inhibits the activity of the promoter for the DNA of the present invention, It can greatly contribute to investigating the cause of various diseases caused or developing preventive and therapeutic agents.
Further, using a DNA containing the promoter region of the protein of the present invention, genes encoding various proteins are ligated downstream thereof and injected into egg cells of an animal to produce a so-called transgenic animal (gene-transferred animal). Once created, it will also be possible to specifically synthesize the protein and study its effects in living organisms. Furthermore, if a suitable reporter gene is bound to the above promoter portion, and a cell line that expresses the reporter gene is established, a low-molecular compound having an action of specifically promoting or suppressing the production ability of the protein itself of the present invention in the body. Can be used as a search system.
[0071]
In the present specification, bases, amino acids, and the like are represented by abbreviations based on the abbreviations by IUPAC-IUB Commission on Biochemical Nomenclature or abbreviations commonly used in the art, and examples thereof are described below. When an amino acid can have an optical isomer, the L-form is indicated unless otherwise specified.
DNA: deoxyribonucleic acid
cDNA: complementary deoxyribonucleic acid
A: Adenine
T: Thymine
G: Guanine
C: Cytosine
RNA: ribonucleic acid
mRNA: messenger ribonucleic acid
dATP: deoxyadenosine triphosphate
dTTP: deoxythymidine triphosphate
dGTP: deoxyguanosine triphosphate
dCTP: deoxycytidine triphosphate
ATP: Adenosine triphosphate
EDTA: Ethylenediaminetetraacetic acid
SDS: Sodium dodecyl sulfate
Gly: glycine
Ala: Alanine
Val: Valine
Leu: Leucine
Ile: Isoleucine
Ser: Serine
Thr: Threonine
Cys: cysteine
Met: methionine
Glu: glutamic acid
Asp: Aspartic acid
Lys: lysine
Arg: Arginine
His: histidine
Phe: phenylalanine
Tyr: Tyrosine
Trp: Tryptophan
Pro: Proline
Asn: Asparagine
Gln: Glutamine
pGlu: pyroglutamic acid
Sec: selenocysteine
[0072]
Further, substituents, protecting groups and reagents frequently used in the present specification are represented by the following symbols.

[0073]
The sequence numbers in the sequence listing in the present specification indicate the following sequences.
[SEQ ID NO: 1]
2 shows the amino acid sequence of human nmb.
[SEQ ID NO: 2]
This shows the base sequence of DNA encoding human nmb having the amino acid sequence represented by SEQ ID NO: 1.
[SEQ ID NO: 3]
1 shows the amino acid sequence of mouse dendritic cell-associated transmembrane protein (DC-HIL).
[SEQ ID NO: 4]
This shows the nucleotide sequence of DNA encoding mouse DC-HIL having the amino acid sequence represented by SEQ ID NO: 3.
[SEQ ID NO: 5]
3 shows the nucleotide sequences of primers used in Examples 2 and 3.
[SEQ ID NO: 6]
3 shows the nucleotide sequences of primers used in Examples 2 and 3.
[SEQ ID NO: 7]
3 shows the nucleotide sequences of primers used in Examples 2 and 3.
[SEQ ID NO: 8]
3 shows the nucleotide sequences of primers used in Examples 2 and 3.
[0074]
Hereinafter, the present invention will be more specifically described with reference to examples, but the present invention is not limited thereto.
【Example】
Example 1
(1) Production of COPD model mouse exposed to cigarette smoke
The COPD model was produced by inhaling mainstream smoke generated from Kentucky Reference Cigarette 1R1 into C57BL / 6N mice (6 weeks old, Charles River Japan) for 1 to 4 hours / day, 5 days / week for a total of 6 months. . That is, the Kentucky Reference Cigarette 1R1 was attached to a cigarette smoke generator (SG-200, Shibata Scientific Co., Ltd.), and mainstream smoke was collected under the conditions of 35 ml / puff, 10 puff / min, and 25 puff / cigarette. After the obtained mainstream smoke was diluted to 3% (V / V) with air, the air was sent to an acrylic exposure chamber containing the mouse, and the mouse under spontaneous breathing was allowed to inhale cigarette smoke for a predetermined time. In addition, normal mice were used for the control group. Mouse lung function was evaluated using a pressure-volume curve of the isolated lung. That is, the mice were anesthetized with pentobarbital (70 mg / kg, ip) on the day after the end of the one-month, three-month and six-month tobacco smoke exposures, and then the neck was incised and the trachea was cannulated. (Surflow indwelling needle, 18G) was inserted. A ventilator (Harvard) was connected to the tracheal cannula and, under diaphragmectomy, 99.995% O 2. ₂ For 10 minutes. The change in airway pressure at that time was 10 cm H ₂ The ventilation was adjusted to be O. After the end of the artificial respiration, the trachea was closed with an arterial clip to perform degassing in the lung, and then the lung was removed. 0 to 25 cm H ₂ Formalin buffer was sequentially injected at a pressure of O and 5 cm H ₂ The lung volume for each O was measured using prethysmograph (Ugobasil), and the pressure-volume curve of the isolated lung was determined. The results are shown in FIG.
[0075]
(2) Search for genes whose expression fluctuates in the lungs of COPD model mice exposed to cigarette smoke
To elucidate the genes whose expression is fluctuated specifically in the lungs of COPD model mice exposed to cigarette smoke, the mice were sacrificed by pentobarbital anesthesia the day after the final exposure, and the lungs were removed after bronchoalveolar lavage did. The excised lung was frozen in liquid nitrogen, crushed by a frozen tissue crusher, and then immersed in Isogen (manufactured by Wako Pure Chemical Industries, Ltd.) corresponding to 10 times its wet weight. 1 month tobacco smoke exposure group (n = 10), its control group (n = 6), 3 month tobacco smoke exposure group (n = 8), its control group (n = 8), 6 month tobacco smoke exposure group (n = 8), total RNA extracted from the control group (n = 8) using ISOGEN according to the attached manual as a material, and expression analysis using oligonucleotide microarray (Mouse Genome U94A, U94B, U94C; Affymetrix) Was done.
The experimental method was in accordance with Affymetrix's Experimental Manual (Expression analysis technical manual). As a result, as a gene whose expression is specifically increased in a COPD model mouse exposed to cigarette smoke, affymetrix No. 108822_at was detected. When a BLAST search was performed based on this sequence, the gene encoded a mouse dendritic cell-associated transmembrane protein (DC-HIL) (sometimes referred to as mouse nmb). The human counterpart was found to be human nmb (SEQ ID NO: 1).
[0076]
Example 2
Confirmation of expression fluctuation by quantitative RT-PCR method
In order to confirm that the expression fluctuation of the DC-HIL gene was remarkably observed even at the individual level, the expression of each individual was examined by a quantitative RT-PCR method.
Using 200 ng of total RNA prepared from mouse lung tissue as a starting material, cDNA was synthesized by a reverse transcription reaction in a 50 μl reaction solution using TaqMan Gold RT-PCR Kit (manufactured by Applied Biosystems). After diluting the reaction solution five-fold with distilled water, 7 μl of the diluted solution was used for real-time quantitative PCR using ABI PRISM 7900 Sequence Detector (manufactured by Applied Biosystems) and QuantiTect SYBR Green PCR Kit (manufactured by QIAGEN). As a result, the copy number of the mouse DC-HIL gene was measured. The primers [Primer 1 (SEQ ID NO: 5) and Primer 2 (SEQ ID NO: 6)] used for the detection of the gene amount were designed using the Primer Express program from the nucleotide sequence of the mouse DC-HIL gene [GenBank Accession Number: AF322054]. did. As a standard sample for calculating the copy number, RT-PCR was performed using primer 3 (SEQ ID NO: 7) and primer 4 (SEQ ID NO: 8) with total RNA extracted from mouse lung tissue as a template. It was prepared by measuring the concentration of a DNA fragment consisting of 515 base pairs by using a Spectrophotometer (manufactured by Beckman) and serially diluting it. Similarly, the copy number of the GAPDH gene was measured as a housekeeping gene. Samples containing no reverse transcriptase were treated in the same manner to remove non-specific amplification, and the number of gene copies per total RNA was calculated from the following formula. Was compared for each individual.
(DC-HIL gene copy number in sample containing reverse transcriptase / GAPDH gene copy number)-(DC-HIL gene copy number / GAPDH gene copy number in sample not containing reverse transcriptase) = (DC-HIL gene expression level) )
FIG. 2 shows the results.
From this, it was found that the expression of the mouse DC-HIL gene (SEQ ID NO: 4) was significantly increased in the lungs of the COPD model mouse (** p ≦ 0.01).
[0077]
Example 3
Analysis of tissue distribution of mouse DC-HIL gene product
Mouse cDNA (Mouse MTC panel I and Mouse MTC panel II: Clontech) and cigarettes of mouse tissues (bone marrow, smooth muscle, prostate, thymus, stomach, uterus, heart, brain, spleen, lung, liver, kidney, testis) Using ABI PRISM 7900 Sequence Detector (manufactured by Applied Biosystems) and QuantiTect SYBR Green PCR Kit (manufactured by QIAGEN) with the smoke-exposed model mouse lung cDNA and control mouse lung cDNA (mixed group treated for 1, 3, 6 months) as templates Mouse DC-HIL gene expression distribution was examined by real-time quantitative PCR. The primers [Primer 1 (SEQ ID NO: 5) and Primer 2 (SEQ ID NO: 6)] used for the detection of the gene amount were designed using the Primer Express program from the nucleotide sequence of the mouse DC-HIL gene [GenBank Accession Number: AF322054]. did. As a standard sample for calculating the copy number, RT-PCR was performed using primer 3 (SEQ ID NO: 7) and primer 4 (SEQ ID NO: 8) with total RNA extracted from mouse lung tissue as a template. It was prepared by measuring the concentration of a DNA fragment consisting of 515 base pairs by using a Spectrophotometer (manufactured by Beckman) and serially diluting it. Similarly, the copy number of the GAPDH gene was measured as a housekeeping gene. In addition, a sample containing no reverse transcriptase was treated in the same manner to remove non-specific amplification, and the expression level was determined by calculating the gene copy number per total RNA according to the following equation.
(DC-HIL gene copy number in sample containing reverse transcriptase / GAPDH gene copy number)-(DC-HIL gene copy number / GAPDH gene copy number in sample not containing reverse transcriptase) = (DC-HIL gene expression level) )
The results are shown in FIG.
As a result, it was found that the mouse DC-HIL gene product (mRNA) was specifically expressed in the lung.
[0078]
Example 4
(1) Preparation of elastase-induced COPD model mouse
The COPD model was prepared by instilling porcine pancreatic elastase solution (Wako Pure Chemical Industries, Ltd.) (6 units / 50 μL / mouse) into C57BL / 6N mice (8 weeks old, Charles River Japan) under halothane anesthesia. In addition, a physiological saline solution nasal mouse was used for the control group. Mouse lung function was evaluated using a pressure-volume curve of the isolated lung. That is, mice were anesthetized with pentobarbital (70 mg / kg intraperitoneally) 1 day, 3 days, 7 days, 14 days, 21 days and 35 days after elastase administration, and then the neck was incised and the trachea was cannulated (surflow). Indwelling needle, 18G) was inserted. A ventilator (Harvard) was connected to the tracheal cannula and 99.995% O 2 was obtained under diaphragmectomy. ₂ Was used for 10 minutes for artificial respiration. The airway load pressure at that time was 10 cm H ₂ The ventilation was adjusted to be O. After the end of the artificial respiration, the trachea was closed with an arterial clip to perform degassing in the lung, and then the lung was removed. 0 to 25 cm H ₂ Under a load pressure of O, formalin buffer was sequentially injected and 5 cm H ₂ The volume of the lung for each O was measured using plethysmograph (manufactured by Ugobasil), and the pressure-volume curve of the removed lung was determined. In addition, a compliance value was calculated as an index of the ease with which the lungs spread according to the following equation.
｛25 cm H ₂ Lung volume increase under load pressure of O (mL)｝ / 25 (cmH ₂ O) = Compliance value
The results are shown in FIGS.
(2) Search for genes whose expression fluctuates in lungs of elastase-induced COPD model mouse
Elastase-induced COPD model To elucidate the gene whose expression is fluctuated specifically in the lung of the mouse, mice were sacrificed by pentobarbital anesthesia 1, 3, 7, 14, 21 and 35 days after elastase administration. The lung was removed. The removed lung was frozen in liquid nitrogen, crushed with a frozen tissue crusher, and then immersed in ISOGEN (Wako Pure Chemical Industries) equivalent to 10 times its wet weight. 1 day after elastase administration, 3 days after elastase administration, 7 days after elastase administration, 14 days after elastase administration, 21 days after elastase administration, 35 days after elastase administration (all n = 6) and their control groups (all n = 6), total RNA was prepared using ISOGEN according to the attached manual.
Using 1 μg of total RNA prepared from mouse lung tissue as a starting material, cDNA was synthesized by reverse transcription in a 50 μl reaction solution using M-MLV Reverse Transcriptase (manufactured by Invitrogen). Using the reaction solution, the amount of mouse DC-HIL gene was measured by a real-time quantitative PCR method using an ABI PRISM 7700 sequence detector (manufactured by Applied Biosystems). The primers [Primer 1 (SEQ ID NO: 5) and Primer 2 (SEQ ID NO: 6)] used for the detection of the gene amount were designed using the Primer Express program from the nucleotide sequence of the mouse DC-HIL gene (GenBank Accession Number: AF322054). did. Similarly, the amount of the 18S ribosomal RNA gene as a housekeeping gene was measured. The DC-HIL gene expression amount per 18S ribosomal RNA gene expression amount was determined from the following formula, and the expression of elastase-induced COPD model mouse lung and control mouse lung was compared for each individual.
(DC-HIL gene expression amount / 18S ribosomal RNA gene expression amount) = (DC-HIL gene expression amount)
FIG. 6 shows the results.
From this, it was found that the expression of the DC-HIL gene (SEQ ID NO: 4) was significantly increased (** p ≦ 0.01) in the lung of the elastase-induced COPD model mouse.
[0079]
【The invention's effect】
The proteins and polynucleotides of the present invention include, for example, respiratory diseases [eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, lung fibrosis Disease), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry pronasitis, vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immunology Diseases (eg, associated with myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistance diabetes, rheumatoid arthritis, systemic lupus erythematosus, atopic dermatitis, leukocyte abnormalities, splenic dysfunction or thymic abnormalities Immunodeficiency, etc.), inflammatory bowel disease, allergic conjunctivitis, etc., and useful as diagnostic markers, etc., for the protein, polynucleotide or the protein. Regulatory agents (preferably inhibitors) obtained by screening using antibodies and the like, neutralizing antibodies against the protein, etc. include, for example, respiratory diseases [eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), Bronchiolitis, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (eg, allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, pre-dryness) Rhinitis, vasomotor rhinitis, gangrenous rhinitis, sinusitis, etc., immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic For the prevention and treatment of lupus erythematosus, atopic dermatitis, leukocyte abnormalities, immunodeficiency associated with spleen dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis, etc. It is possible to use. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
In addition, the antisense polynucleotide of the present invention can suppress the expression of the protein of the present invention. Examples thereof include respiratory diseases (eg, chronic obstructive pulmonary disease (chronic bronchitis, emphysema), diffuse panbronchiolosis). Inflammation, bronchial asthma, cystic fibrosis, irritable pneumonia, pulmonary fibrosis, etc.), rhinitis (e.g., allergic rhinitis, hay fever, acute rhinitis, chronic rhinitis, hypertrophic rhinitis, atrophic rhinitis, dry pronasitis, Vasomotor rhinitis, gangrene rhinitis, sinusitis, etc.), immune disorders (eg, myasthenia gravis, glomerulonephritis, multiple sclerosis, Sjogren's syndrome, insulin resistant diabetes, rheumatoid arthritis, systemic lupus erythematosus, Atopic dermatitis, leukocyte abnormalities, immunodeficiency due to spleen dysfunction or thymic abnormalities), inflammatory bowel disease, allergic conjunctivitis, etc. Can. Preferably, it is a prophylactic / therapeutic agent for a respiratory disease or the like, more preferably a prophylactic / therapeutic agent for a chronic obstructive pulmonary disease or the like, and further preferably a prophylactic / therapeutic agent for a pulmonary emphysema or the like.
[0080]
[Sequence list]

[Brief description of the drawings]
FIG. 1 is a diagram showing a pressure-volume curve of an isolated mouse lung obtained in Example 1. In the figure,-●-in (a) represents a group of mice exposed to cigarette smoke for one month (n = 8),-○-represents a control group (n = 7), and-●-in (b) represents three months. Group of mice exposed to cigarette smoke (n = 10),-○-represents the control group (n = 9), and-●-in (c) represents the group of mice exposed to tobacco smoke for 6 months (n = 10), -− -Indicates a control group (n = 9). ** indicates p ≦ 0.01, and * indicates p ≦ 0.05.
FIG. 2 is a diagram showing the results of mouse DC-HIL gene expression levels obtained in Example 2. In the figure, A represents the lung of a mouse exposed to cigarette smoke for 1 month, B represents the lung of a control mouse, C represents the lung of a mouse exposed to cigarette smoke for 3 months, D represents the lung of the control mouse, and E represents the lung of 6 months. The lung of a mouse exposed to tobacco smoke, F indicates the control mouse lung.
FIG. 3 is a diagram showing the results of mouse DC-HIL gene expression distribution obtained in Example 3.
FIG. 4 is a diagram showing a pressure-volume curve of a mouse extirpated lung obtained in Example 4. In the figure,-■-in (a) represents the mouse group (n = 6) one day after elastase administration,-□-represents the control group (n = 6), and (b)-■-represents the mouse group 7 days after elastase administration. Model mouse group (n = 5),-□-represents control group (n = 6), (c)-（-represents model mouse group 21 days after elastase administration (n = 6),-□-represents control group (N = 6). * Indicates p ≦ 0.05, and ** indicates p ≦ 0.01.
FIG. 5 is a graph showing the change over time in the compliance value of the isolated lung of a mouse after administration of elastase obtained in Example 4. In the figure, the horizontal axis indicates the number of days after elastase administration, and the vertical axis indicates the compliance value. -■-indicates an elastase-administered mouse group (n = 6), and-□-indicates a control group (n = 6). * Indicates p ≦ 0.05, and ** indicates p ≦ 0.01.
FIG. 6 is a graph showing the time-course change of the expression level of DC-HIL gene in mouse lung tissue after elastase administration obtained in Example 4. In the figure, the horizontal axis indicates the number of days after elastase administration, and the vertical axis indicates the DC-HIL gene expression level. -■-indicates an elastase-administered mouse group (n = 6), and-□-indicates a control group (n = 6). * Indicates p ≦ 0.05, and ** indicates p ≦ 0.01.

Claims (25)

Prevention of a respiratory disease comprising a compound having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof or a compound inhibiting the activity of a salt thereof or a salt thereof -Therapeutic agents. A respiratory disease comprising a compound having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a compound inhibiting the expression of a salt gene or a salt thereof Prophylactic and therapeutic agents. A nucleotide sequence complementary or substantially complementary to the nucleotide sequence of a polynucleotide encoding a protein or a partial peptide thereof containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, or An antisense polynucleotide containing a portion. A medicament comprising the antisense polynucleotide according to claim 3. The medicament according to claim 4, which is an agent for preventing or treating respiratory diseases. An antibody against a protein containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof. A medicament comprising the antibody according to claim 6. The medicament according to claim 7, which is an agent for preventing or treating respiratory diseases. A diagnostic agent comprising the antibody according to claim 6. The diagnostic agent according to claim 9, which is a diagnostic agent for a respiratory disease. A diagnostic agent for a respiratory disease comprising a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof. A prophylactic / therapeutic agent for a respiratory disease comprising a compound having an action of inhibiting heparan sulfate proteoglycan binding activity or a salt thereof. A method for screening a prophylactic / therapeutic agent for a respiratory disease, which comprises using a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof. 14. The screening method according to claim 13, wherein a chronic obstructive pulmonary disease model mouse or an elastase-induced chronic obstructive pulmonary disease model mouse is used. For screening a prophylactic / therapeutic agent for a respiratory disease, comprising a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, or a partial peptide thereof or a salt thereof. kit. An agent for preventing or treating respiratory diseases obtainable by using the screening method according to claim 13 or the screening kit according to claim 15. 17. The prophylactic / therapeutic agent according to claim 16, wherein the respiratory disease is emphysema. Screening of a preventive / therapeutic agent for a respiratory disease, characterized by using a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof. Method. 19. The screening method according to claim 18, wherein a tobacco smoke-exposed chronic obstructive pulmonary disease model mouse or an elastase-induced chronic obstructive pulmonary disease model mouse is used. A preventive / therapeutic agent for a respiratory disease comprising a polynucleotide encoding a protein having the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof. Screening kit. An agent for preventing or treating respiratory diseases obtainable by using the screening method according to claim 18 or the screening kit according to claim 20. The prophylactic / therapeutic agent according to claim 21, wherein the respiratory disease is emphysema. A compound that inhibits the activity of a protein containing an amino acid sequence identical or substantially identical to the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof or a salt thereof, or a salt thereof, A method for preventing or treating respiratory diseases, which comprises administering an effective amount of a compound that inhibits gene expression or a salt thereof. Inhibits the activity of a protein containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1, a partial peptide thereof, or a salt thereof, or inhibits the expression of a gene of the protein Prevention and treatment method for respiratory diseases. Inhibits the activity of a protein containing the same or substantially the same amino acid sequence as the amino acid sequence represented by SEQ ID NO: 1 or a partial peptide thereof or a salt thereof for producing a prophylactic / therapeutic agent for a respiratory disease Use of a compound or a salt thereof, or a compound or a salt thereof that inhibits expression of a gene of the protein.

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